Grading of breast cancer

ABSTRACT

Methods and compositions for the identification of breast cancer grade signatures are provided. The signature profiles are identified based upon multiple sampling of reference breast tissue samples from independent cases of breast cancer and provide a reliable set of molecular criteria for identification of cells as being in one or more particular stages and/or grades of breast cancer.

CROSS-REFERENCE TO RELATED APPLICATIONS

This application is a continuation of application Ser. No. 13/083,500, filed Apr. 8, 2011, which is a continuation of U.S. patent application Ser. No. 11/946,835, filed Nov. 28, 2007, now U.S. Pat. No. 7,930,105, which is a continuation of U.S. patent application Ser. No. 10/211,015, filed Aug. 1, 2002, which is a continuation-in-part of U.S. Pat. No. 10/028,018, filed Dec. 21, 2001, the disclosures of each of which are incorporated herein by reference as if fully set forth.

FIELD OF THE INVENTION

The invention relates to the identification and use of gene expression profiles, or patterns, involved in breast cancer progression. In particular, the invention provides the identities of genes that may be used to identify different grades of breast cancer within and between stages thereof. The gene expression profiles, whether embodied in nucleic acid expression, protein expression, or other expression formats, are used in the study and/or diagnosis of cells and tissue during breast cancer progression as well as for the study and/or determination of prognosis of a patient. When used for diagnosis or prognosis, the profiles are used to predict the status and/or phenotype of cells and tissues relative to breast cancer and the treatment thereof.

BACKGROUND OF THE INVENTION

Breast cancer is by far the most common cancer among women. Each year, more than 180,000 and 1 million women in the U.S. and worldwide, respectively, are diagnosed with breast cancer. Breast cancer is the leading cause of death for women between ages 50-55, and is the most common non-preventable malignancy in women in the Western Hemisphere. An estimated 2,167,000 women in the United States are currently living with the disease (National Cancer Institute, Surveillance Epidemiology and End Results (NCI SEER) program, Cancer Statistics Review (CSR), www-seer.ims.nci.nih.gov/Publications/CSR1973 (1998)). Based on cancer rates from 1995 through 1997, a report from the National Cancer Institute (NCI) estimates that about 1 in 8 women in the United States (approximately 12.8 percent) will develop breast cancer during her lifetime (NCI's Surveillance, Epidemiology, and End Results Program (SEER) publication SEER Cancer Statistic's Review 1973-1997). Breast cancer is the second most common form of cancer, after skin cancer, among women in the United States. An estimated 250,100 new cases of breast cancer are expected to be diagnosed in the United States in 2001. Of these, 192,200 new cases of more advanced (invasive) breast cancer are expected to occur among women (an increase of 5% over last year), 46,400 new cases of early stage (in situ) breast cancer are expected to occur among women (up 9% from last year), and about 1,500 new cases of breast cancer are expected to be diagnosed in men (Cancer Facts & FIGS. 2001 American Cancer Society). An estimated 40,600 deaths (40,300 women, 400 men) from breast cancer are expected in 2001. Breast cancer ranks second only to lung cancer among causes of cancer deaths in women. Nearly 86% of women who are diagnosed with breast cancer are likely to still be alive five years later, though 24% of them will die of breast cancer after 10 years, and nearly half (47%) will die of breast cancer after 20 years.

Every woman is at risk for breast cancer. Over 70 percent (Abreast cancers occur in women who have no identifiable risk factors other than age (U.S. General Accounting Office. Breast Cancer, 1971-1991: Prevention, Treatment and Research. GAO/PEMD-92-12; 1991). Only 5 to 10% of breast cancers are linked to a family history of breast cancer (Henderson I C, Breast Cancer. In: Murphy G P, Lawrence W L, Lenhard R E (eds). Clinical Oncology. Atlanta, Ga.: American Cancer Society; 1995:198-219).

Each breast has 15 to 20 sections called lobes. Within each lobe are many smaller lobules. Lobules end in dozens of tiny bulbs that can produce milk. The lobes, lobules, and bulbs are all linked by thin tubes called ducts. These ducts lead to the nipple in the center of a dark area of skin called the areola. Fat surrounds the lobules and ducts. There are no muscles in the breast, but muscles lie under each breast and cover the ribs. Each breast also contains blood vessels and lymph vessels. The lymph vessels carry colorless fluid called lymph, and lead to the lymph nodes. Clusters of lymph nodes are found near the breast in the axilla (under the arm), above the collarbone, and in the chest.

Breast tumors can be either benign or malignant. Benign tumors are not cancerous, they do not spread to other parts of the body, and are not a threat to life. They can usually be removed, and in most cases, do not come back. Malignant tumors are cancerous, and can invade and damage nearby tissues and organs. Malignant tumor cells may metastasize, entering the bloodstream or lymphatic system. When breast cancer cells metastasize outside the breast, they are often found in the lymph nodes under the arm (axillary lymph nodes). If the cancer has reached these nodes, it means that cancer cells may have spread to other lymph nodes or other organs, such as bones, liver, or lungs.

Major and intensive research has been focussed on early detection, treatment and prevention. This has included an emphasis on determining the presence of precancerous or cancerous ductal epithelial cells. These cells are analyzed, for example, for cell morphology, for protein markers, for nucleic acid markers, for chromosomal abnormalities, for biochemical markers, and for other characteristic changes that would signal the presence of cancerous or precancerous cells. This has led to various molecular alterations that have been reported in breast cancer, few of which have been well characterized in human clinical breast specimens. Molecular alterations include presence/absence of estrogen and progesterone steroid receptors, HER-2 expression/amplification (Mark H F, et al. HER-2/neu gene amplification in stages I-IV breast cancer detected by fluorescent in situ hybridization. Genet Med; 1(3):98-103 1999), Ki-67 (an antigen that is present in all stages of the cell cycle except G0 and used as a marker for tumor cell proliferation, and prognostic markers (including oncogenes, tumor suppressor genes, and angiogenesis markers) like p53, p27, Cathepsin D, pS2, multi-drug resistance (MDR) gene, and CD31.

Examination of cells by a trained pathologist has also been used to establish whether ductal epithelial cells are normal (i.e. not precancerous or cancerous or, having another noncancerous abnormality), precancerous (i.e. comprising hyperplasia, atypical ductal hyperplasia (ADH)) or cancerous (comprising ductal carcinoma in situ, or DCIS, which includes low grade ductal carcinoma in situ, or LG-DCIS, and high grade ductal carcinoma in situ, or HG-DCIS) or invasive (ductal) carcinoma (IDC). Pathologists may also identify the occurrence of lobular carcinoma in situ (LCIS) or invasive lobular carcinoma (ILC). Breast cancer progression may be viewed as the occurrence of abnormal cells, such as those of ADH, DCIS, IDC, LCIS, and/or ILC, among normal cells.

It remains unclear whether normal cells become hyperplastic (such as ADH) and then progressing on to become malignant (DCIS, IDC, LCIS, and/or ILC) or whether normal cells are able to directly become malignant without transitioning through a hyperplastic stage. It has been observed, however, that the presence of ADH indicates a higher likelihood of developing a malignancy. This has resulting in treatment of patients with ADH to begin treatment with an antineoplastic/antitumor agent such as tamoxifen. This is in contrast to the treatment of patients with malignant breast cancer which usually includes surgical removal.

The rational development of preventive, diagnostic and therapeutic strategies for women at risk for breast cancer would be aided by a molecular map of the tumorigenesis process. Relatively little is known of the molecular events that mediate the transition of normal breast cells to the various stages of breast cancer progression. Similarly, little is known of the molecular events that mediate the transition of cells from one stage of breast cancer to another.

Molecular means of identifying the differences between normal, non-cancerous cells and cancerous cells (in general) have been the focus of intense study. The use of cDNA libraries to analyze differences in gene expression patterns in normal versus tumorigenic cells has been described (U.S. Pat. No. 4,981,783). DeRisi et al. (1996) describe the analysis of gene expression patterns between two cell lines: UACC-903, which is a tumorigenic human melanoma cell line, and UACC-903(+6), which is a chromosome 6 suppressed non-tumorigenic form of UACC-903. Labeled cDNA probes made from mRNA from these cell lines were applied to DNA microarrays containing 870 different cDNAs and controls. Genes that were preferentially expressed in one of the two cell lines were identified.

Golub et al. (1999) describe the use of gene expression monitoring as means to cancer class discovery and class prediction between acute myeloid leukemia (AML) and acute lymphoblastic leukemia (ALL). Their approach to class predictors used a neighborhood analysis followed by cross-validation of the validity of the predictors by withholding one sample and building a predictor based only on the remaining samples. This predictor is then used to predict the class of the withheld sample. They also used cluster analysis to identify new classes (or subtypes) within the AML and ALL.

Gene expression patterns in human breast cancers have been described by Perou et al. (1999), who studied gene expression between cultured human mammary epithelia cells (HMEC) and breast tissue samples by use of microarrays comprising about 5000 genes. They used a clustering algorithm to identify patterns of expression in HMEC and tissue samples. Peron et al. (2000) describe the use of clustered gene expression profiles to classify subtypes of human breast tumors. Hedenfalk et al. describe gene expression profiles in BRCA1 mutation positive, BRCA2 mutation positive, and sporadic tumors. Using gene expression patterns to distinguish breast tumor subclasses and predict clinical implications is described by Sortie et al. and West et al.

All of the above described approaches, however, utilize heterogeneous populations of cells found in culture or in a biopsy to obtain information on gene expression patterns. The use of such populations may result in the inclusion or exclusion of multiple genes from the patterns. For this and the lack of statistical robustness reasons, the gene expression patterns observed by the above described approaches provide little confidence that the differences in gene expression may be meaningfully associated with the stages of breast cancer.

Citation of documents herein is not intended as an admission that any is pertinent prior art. All statements as to the date or representation as to the contents of documents is based on the information available to the applicant and does not constitute any admission as to the correctness of the dates or contents of the documents.

SUMMARY OF THE INVENTION

The present invention relates to the identification and use of gene expression patterns (or profiles or “signatures”) which are correlated with (and thus able to discriminate between) cells in various stages and/or grades of breast cancer. Broadly defined, these stages are non-malignant versus malignant, but may also be viewed as normal versus atypical (optionally including reactive and pre-neoplastic) versus cancerous. Another definition of the stages is normal versus precancerous (e.g. atypical ductal hyperplasia (ADH) or atypical lobular hyperplasia (ALH)) versus cancerous (e.g. carcinoma in situ such as DCIS and/or LCIS) versus invasive (e.g. carcinomas such as IDC and/or ILC). The invention may also be applied to discriminations between normal and non-normal (including cancerous and other non-normal cells).

The invention also relates to the identification and use of gene expression patterns (or profiles or “signatures”) which are correlated with (and thus able to discriminate between) cells in various grades (within one or more stage) of breast cancer. Grading of breast cancer is normally done for cases of invasive ductal carcinoma (IDC), and may be done for invasive lobular carcinoma (ILC) as well, where cytological criteria such as the Nottingham BSR, nuclear morphology, tissue architecture, proliferation index (such as assays for PCNA or Ki67), and extent of differentiation are used to assign a grade of I, II or III to particular breast cancer samples. Grade I is usually where the cells are still well differentiated and are usually positive for the estrogen receptor (ER). Grade III is usually where the cells are poorly differentiated and usually negative for ER. Grade II is generally where the cells have characteristics intermediate between grades I and III and can make up approximately 60% of all samples assayed. This is rather unfortunate because determination of grade in IDC is used directly for decisions on patient care.

Grading of cases of ductal carcinoma in situ (DCIS) is also possible, but is not routine in current clinical practice. Grading of lobular carcinoma in situ (LCIS) is also possible. In addition to grades I to III, conventional grading schemes may use the terms “tow grade” and/or “high grade.”

The present invention provides a non-subjective means for the identification of grades of various stages of cancer by assaying for the expression patterns associated with particular grades. Thus where subjective interpretation is used in grade assessment by pathologists using cytological criteria, the present invention provides objective gene expression patterns, which may optionally be performed in the absence of grading by histomorphological or cytological criteria, that are correlated with grades (or low to high grade) to provide a more accurate assessment of breast cancer progression. The expression patterns of the invention thus provide a means to determine breast cancer prognosis. Furthermore, the expression patterns can also be used as a means to assay small, node negative tumors that are not readily graded by conventional means.

The gene expression patterns comprise one or more than one gene capable of discriminating between various stages and/or grades of breast cancer with significant accuracy. The gene(s) are identified as correlated with various stages and/or grades of breast cancer such that the levels of their expression are relevant to a determination of the stage and/or grade of breast cancer of a cell. Thus in one aspect, the invention provides a method to determine the stage and/or grade of breast cancer of a subject afflicted with, or suspected of having, breast cancer by assaying a cell containing sample from said subject for expression clone or more than one gene disclosed herein as correlated with one or more stages and/or grades of breast cancer.

Gene expression patterns of the invention are identified by analysis of gene expression in multiple samples of each stage and/or grade to be studied. The overall gene expression profile of a sample is obtained through quantifying the expression levels of mRNA corresponding to approximately 12000 genes. This overall profile is then analyzed to identify genes that are positively, or negatively, correlated, with a stage and/or grade of breast cancer. An expression profile of a subset of human genes may then be identified by the methods of the present invention as correlated with a particular stage and/or grade of breast cancer. The use of multiple samples increases the confidence which a gene may be believed to be correlated with a particular stage and/or grade. Without sufficient confidence, it remains unpredictable whether a particular gene is actually correlated with a stage and/or grade of breast cancer and also unpredictable whether a particular gene may be successfully used to identify the stage and/or grade of an unknown breast cancer cell sample.

A profile of genes that are highly correlated with one stage and/or grade relative to another may be used to assay an sample from a subject afflicted with, or suspected of having, breast cancer to identify the stage and/or grade of breast cancer to which the sample belongs. Such an assay may be used as part of a method to determine the therapeutic treatment for said subject based upon the stage(s) and/or grade(s) of breast cancer identified. The present invention thus also provides for the advantageous ability to determine grade of a stage of breast cancer in combination with stage information to provide more detailed information in diagnosing and treating breast cancer. This has not always been possible in the diagnosis and treatment of breast cancer using previous protocols, where it was often only possible to determine stage with grade being only occasionally determinable.

The correlated genes may be used singly with significant accuracy or in combination increase the ability to accurately discriminate between various stages and/or grades of breast cancer. The present invention thus provides means tar correlating a molecular expression phenotype with a physiological (cellular) stage or state. This correlation provides a way to molecularly diagnose and/or monitor a cells status in comparison to different cancerous versus non-cancerous phenotypes as disclosed herein. Additional uses of the correlated gene(s) are in the classification of cells and tissues; determination of diagnosis and/or prognosis; and determination and/or alteration of therapy.

The ability to discriminate is conferred by the identification of expression of the individual genes as relevant and not by the form of the assay used to determine the actual level of expression. An assay may utilize any identifying feature of an identified individual gene as disclosed herein as long as the assay reflects, quantitatively or qualitatively, expression of the gene. Identifying features include, but are not limited to, unique nucleic acid, sequences used to encode (DNA), or express (RNA), said gene or epitopes specific to, or activities of, a protein encoded by said gene. All that is required is the identity of the gene(s) necessary to discriminate between stages and/or grades of breast cancer and an appropriate cell containing sample for use in an expression assay.

In one aspect, the invention provides for the identification of the gene expression patterns by analyzing global, or near global, gene expression from single cells or homogenous cell populations which have been dissected away from, or otherwise isolated or purified from, contaminating cells beyond that possible by a simple biopsy. Because the expression of numerous genes fluctuate between cells from different patients as well as between cells from the same patient sample, multiple individual gene expression patterns are used as reference data to generate models which in turn permit the identification of individual gene(s) that are most highly correlated with particular breast cancer stages, and/or grades, and/or have the best the ability to discriminate cells of one stage and/or grade from another.

Use of the present invention has resulted in the identification of two major changes in gene expression, one of which is associated with the transition of normal breast cells to ADH (and persisting in a majority of DCIS and IDC cells), and the second is associated with tumor grade progression. The invention also provides the identification of a subset of genes that differ quantitatively in expression between DCIS and IDC cells.

In another aspect, the invention provides physical and methodological means for detecting the expression of gene(s) identified by the models generated by individual expression patterns. These means may be directed to assaying one or more aspect of the DNA template(s) underlying the expression of the gene(s), of the RNA used as an intermediate to express the gene(s), or of the proteinaceous product expressed by the gene(s).

In a further aspect, the gene(s) identified by a model as capable of discriminating between breast cancer stages and/or grades may be used to identify the cellular state of an unknown sample of cell(s) from the breast. Preferably, the sample is isolated via non-invasive means. The expression of said gene(s) in said unknown sample may be determined and compared to the expression of said gene(s) in reference data of gene expression patterns from the various stages and/or grades of breast cancer. Optionally, the comparison to reference samples may be by comparison to the model(s) constructed based on the reference samples.

One advantage provided by the present invention is that contaminating, non-breast cells (such as infiltrating lymphocytes or other immune system cells) are not present to possibly affect the genes identified or the subsequent analysis of gene expression to identify the status of suspected breast cancer cells. Such contamination is present where a biopsy is used to generate gene expression profiles.

While the present invention has been described mainly in the context of human breast cancer, it may be practiced in the context of breast cancer of any animal known to be potentially afflicted by breast cancer. Preferred animals for the application of the present invention are mammals, particularly those important to agricultural applications (such as, but not limited to, cattle, sheep, horses, and other “farm animals”) and for human companionship (such as, but not limited to, dogs and cats).

BRIEF DESCRIPTION OF THE FIGURES

FIG. 1. Laser capture microdissection. Phenotypically normal breast epithelium and phenotypically abnormal epithelium from atypical ductal hyperplasia (ADH), ductal carcinoma in situ (DCIS) and invasive ductal carcinoma (IDC) from a single breast specimen (case 79) were captured from hematoxylin and eosin-stained sections (8 m in thickness). Panels A, B and C show the images of pre-capture, post-capture, and the captured epithelial compartments, respectively.

FIGS. 2a and 2b . Expression profiles of breast cancer progression. 2 a. Data matrix of 1940 genes by breast cancer samples of different pathological stages. Columns represent samples of tissues identified as ADH; grades I, II, or III of DCIS; and grades I, II, or III of IDC. Rows represent genes. Color scale shown at left bottom. Genes are ordered by hierarchical clustering, and samples are ordered by pathological stage and tumor grade. 2 b. Examples of interesting clusters I, II and III.

FIG. 3. Two-dimensional clustering of 62 samples and 200 genes correlated with tumor grade. Genes (columns) and samples (rows) were clustered independently using a hierarchical clustering algorithm. Red dots indicate ADH samples and green dots indicate grade II samples (DCIS or IDC). Three main clusters (down regulated, Grade III signature, and Grade I signature) are highlighted by color bars. See FIG. 2A for color scale.

FIG. 4. Genes with increased expression in IDC relative to DCIS. Two dimensional clustering was applied to 1688 genes and 24 IDC samples and a portion of the data matrix is shown to highlight a cluster of genes with higher expression in IDC than its corresponding DCIS from the same patient. Expression values are expressed as log-ratios of expression in IDC to that in DCIS. Color scheme shown at left bottom.

FIG. 5. Breast cancer progression model. Breast cancer initiates within normal epithelium evolving into ADH, which progresses into grade I DCIS. A simultaneous 2-dimensional process drives tumor grade progression from I to II to III and stage progression from DCIS to IDC.

DETAILED DESCRIPTION OF THE SPECIFIC EMBODIMENTS

Definitions of terms as used herein:

A gene expression “pattern” or “profile” or “signature” refers to the relative expression of a gene between two or more stages of breast cancer which is correlated with being able to distinguish between said stages.

A “gene” is a polynucleotide that encodes a discrete product, whether RNA or proteinaceous in nature. It is appreciated that more than one polynucleotide may be capable of encoding a discrete product. The term includes alleles and polymorphisms of a gene that encodes the same product, or a functionally associated (including gain, loss, or modulation of function) analog thereof, based upon chromosomal location and ability to recombine during normal mitosis.

A “stage” or “stages” (or equivalents thereof) of breast cancer refer to a physiologic state of a breast cell as defined by known cytological or histological (including immunohistology, histochemistry, and immunohistochemistry) procedures and are readily known to skilled in the art. Non-limiting examples include normal versus abnormal, non-cancerous versus cancerous, the different stages described herein (e.g. hyperplastic, carcinoma, and invasive), and grades within different stages (e.g. grades I, II, or III or the equivalents thereof within cancerous stages).

The terms “correlate” or “correlation” or equivalents thereof refer to an association between expression of one or more genes and a physiologic state of a breast cell to the exclusion of one or more other stages and/or identified by use of the methods as described herein. A gene may be expressed at higher or lower levels and still be correlated with one or more breast cancer stages.

A “polynucleotide” is a polymeric form of nucleotides of any length either ribonucleotides or deoxyribonucleotides. This term refers only to the primary structure of the molecule. Thus, this term includes double- and single-stranded DNA and RNA. It also includes known types of modifications including labels known in the art, methylation, “caps”, substitution of one or more of the naturally occurring nucleotides with an analog, and internucleotide modifications such as uncharged linkages (e.g., phosphorothioates, phosphorodithioates, etc.), as well as unmodified forms of the polynucleotide.

The term “amplify” is used in the broad sense to mean creating an amplification product can be made enzymatically with DNA or RNA polymerases. “Amplification,” as used herein, generally refers to the process of producing multiple copies of a desired sequence, particularly those of a sample. “Multiple copies” mean at least 2 copies. A “copy” does not necessarily mean perfect sequence complementarity or identity to the template sequence.

By corresponding is meant that a nucleic acid molecule shares a substantial amount of sequence identity with another nucleic acid molecule. Substantial amount means at least 95%, usually at least 98% and more usually at least 99%, and sequence identity is determined using the BLAST algorithm, as described in Altschul et al. (1990), J. Mol. Biol. 215:403-410 (using the published default setting, i.e. parameters w=4, t=17). Methods for amplifying mRNA are generally known in the art, and include reverse transcription PCR (RT-PCR) and those described in U.S. patent application Ser. No. 10/062,857 entitled “Nucleic Acid Amplification” filed on Oct. 25, 2001 as well as U.S. Provisional Patent Applications 60/298,847 (filed Jun. 15, 2001) and 60/257,801 (filed Dec. 22, 2000), all of which are hereby incorporated by reference in their entireties as if fully set forth. Another method which may be used is quantitative PCR (or Q-PCR). Alternatively, RNA may be directly labeled as the corresponding cDNA by methods known in the art.

A “microarray” is a linear or two-dimensional array of preferably discrete regions, each having a defined area, formed on the surface of a solid support such as, but not limited to, glass, plastic, or synthetic membrane. The density of the discrete regions on a microarray is determined by the total numbers of immobilized polynucleotides to be detected on the surface of a single solid phase support, preferably at least about 50/cm², more preferably at least about 100/cm², even more preferably at least about 500/cm², but preferably below about 1,000/cm². Preferably, the arrays contain less than about 500, about 1000, about 1500, about 2000, about 2500, or about 3000 immobilized polynucleotides in total. As used herein, a DNA microarray is an array of oligonucleotides or polynucleotides placed on a chip or other surfaces used to hybridize to amplified or cloned polynucleotides from a sample. Since the position of each particular group of primers in the array is known, the identities of a sample polynucleotides can be determined based on their binding to a particular position in the microarray.

Because the invention relies upon the identification of genes that are over- or underexpressed, one embodiment of the invention involves determining expression by hybridization of mRNA, or an amplified or cloned version thereof, of a sample cell to a polynucleotide that is unique to a particular gene sequence. Preferred polynucleotides of this type contain at least about 20, at least about 22, at least about 24, at least about 26, at least about 28, at least about 30, or at least about 32 consecutive basepairs of a gene sequence that is not found in other gene sequences. The term “about” as used in the previous sentence refers to an increase or decrease of 1 from the stated numerical value. Even more preferred are polynucleotides of at least or about 50, at least or about 100, at least about or 150, at least or about 200, at least or about 250, at least or about 300, at least or about 350, or at least or about 400 basepairs of a gene sequence that is not found in other gene sequences. The term “about” as used in the preceding sentence refers to an increase or decrease of 10% from the stated numerical value. Such polynucleotides may also be referred to as polynucleotide probes that are capable of hybridizing to sequences of the genes, or unique portions thereof, described herein. Preferably, the sequences are those of mRNA encoded by the genes, the corresponding cDNA to such mRNAs, and/or amplified versions of such sequences. In preferred embodiments of the invention, the polynucleotide probes are immobilized on an array, other devices, or in individual spots that localize the probes.

Alternatively, and in another embodiment of the invention, gene expression may be determined by analysis of expressed protein in a cell sample of interest by use of one or more antibodies specific for one or more epitopes of individual gene products (proteins) in said cell sample. Such antibodies are preferably labeled to permit their easy detection after binding to the gene product.

The term “label” refers to a composition capable of producing a detectable signal indicative of the presence of the labeled molecule. Suitable labels include radioisotopes, nucleotide chromophores, enzymes, substrates, fluorescent molecules, chemiluminescent moieties, magnetic particles, bioluminescent moieties, and the like. As such, a label is any composition detectable by spectroscopic, photochemical, biochemical, immunochemical, electrical, optical or chemical means.

The term “support” refers to conventional supports such as beads, particles, dipsticks, fibers, filters, membranes and silane or silicate supports such as glass slides.

As used herein, a “breast tissue sample” or “breast cell sample” refers to a sample of breast tissue or fluid isolated from an individual suspected of being afflicted with, or at risk of developing, breast cancer. Such samples are primary isolates (in contrast to cultured cells) and may be collected by any non-invasive means, including, but not limited to, ductal lavage, fine needle aspiration, needle biopsy, the devices and methods described in U.S. Pat. No. 6,328,709, or any other suitable means recognized in the art. Alternatively, the “sample” may be collected by an invasive method, including, but not limited to, surgical biopsy.

“Expression” and “gene expression” include transcription and/or translation of nucleic acid material.

As used herein, the term “comprising” and its cognates are used in their inclusive sense; that is, equivalent to the term, “including” and its corresponding cognates.

Conditions that “allow” an event to occur or conditions that are “suitable” for an event to occur, such as hybridization, strand extension, and the like, or “suitable” conditions are conditions that do not prevent such events from occurring. Thus, these conditions permit, enhance, facilitate, and/or are conducive to the event. Such conditions, known in the art and described herein, depend upon, for example, the nature of the nucleotide sequence, temperature, and buffer conditions. These conditions also depend on what event is desired, such as hybridization, cleavage, strand extension or transcription.

Sequence “mutation,” as used herein, refers to any sequence alteration in the sequence of a gene disclosed herein interest in comparison to a reference sequence. A sequence mutation includes single nucleotide changes, or alterations of more than one nucleotide in a sequence, due to mechanisms such as substitution, deletion or insertion. Single nucleotide polymorphism (SNP) is also a sequence mutation as used herein. Because the present invention is based on the relative level of gene expression, mutations in non-coding regions of genes as disclosed herein may also be assayed in the practice of the invention.

“Detection” includes any means of detecting, including direct and indirect detection of gene expression and changes therein. For example, “detectably less” products may be observed directly or indirectly, and the term indicates any reduction (including the absence of detectable signal). Similarly, “detectably more” product means any increase, whether observed directly or indirectly.

Unless defined otherwise alt technical and scientific terms used herein have the same meaning as commonly understood to one of ordinary skill in the art to which this invention belongs.

Specific Embodiments

The present invention relates to the identification and use of gene expression patterns (or profiles or “signatures”) which discriminate between (or are correlated with) cells in various stages and/or grades of breast cancer. Such patterns may be determined by the methods of the invention by use of a number of reference cell or tissue samples, such as those reviewed by a pathologist of ordinary skill in the pathology of breast cancer, which reflect various stages and/or grades of breast cancer. Because the overall gene expression profile differs from person to person, cancer to cancer, and cancer cell to cancer cell, correlations between certain cell states and genes expressed or underexpressed may be made as disclosed herein to identify genes that are capable of discriminating between different breast cancer states.

The present invention may be practiced with any number of genes believed, or likely to be, differentially expressed in breast cancer cells. Approximately 12,000 genes were used to identify hundreds of genes capable of discriminating between various stages and/or grades of breast cancer as shown in the following Examples. The identification may be made by using expression profiles of various homogenous normal and breast cancer cell populations, which were isolated by microdissection, such as, but not limited to, laser capture microdissection (LCM) of 100-1000 cells. Each gene of the expression profile may be assigned weights based on its ability to discriminate between two or more stages and/or grades of breast cancer. The magnitude of each assigned weight indicates the extent of difference in expression between the two groups and is an approximation of the ability of expression of the gene to discriminate between the two groups (and thus stages and/or grades). The magnitude of each assigned weight also approximates the extent of correlation between expression of individual gene(s) and particular breast cancer stages and/or grades.

It should be noted that merely high levels of expression in cells from a particular stage or grade does not necessarily mean that a gene will be identified as having a high absolute weight value.

Genes with top ranking weights (in absolute terms) may be used to generate models of gene expressions that would maximally discriminate between the two groups. Alternatively, genes with top ranking weights (in absolute terms) may be used in combination with genes with lower weights without significant loss of ability to discriminate between groups. Such models may be generated by any appropriate means recognized in the art, including, but not limited to, cluster analysis, supported vector machines, neural networks or other algorithm known in the art. The models are capable of predicting the classification of a unknown sample based upon the expression of the genes used for discrimination in the models. “Leave one out” cross-validation may be used to test the performance of various models and to help identify weights (genes) that are uninformative or detrimental to the predictive ability of the models. Cross-validation may also be used to identify genes that enhance the predictive ability of the models.

The gene(s) identified as correlated with particular breast cancer stages and/or grades by the above models provide the ability to focus gene expression analysis to only those genes that contribute to the ability to identify a cell as being in a particular stage and/or grade of breast cancer relative to another stage or grade. The expression of other genes in a breast cancer cell would be relatively unable to provide information concerning, and thus assist in the discrimination of, different stages of breast cancer. For example, the cysteine-rich protein 1 (intestinal), identified by I.M.A.G.E. Consortium CloneID 1323448 (“The I.M.A.G.E. Consortium: An Integrated Molecular Analysis of Genomes and their Expression,” Lennon et al., 1996, Genomics 33:151-152; see also image.llnl.gov) has been found to be useful in discriminations between normal and ADH cells (with persistence through DCIS and IDC). Thus expression of this gene would be utilized in models to discriminate between the above listed stages but not for discerning between other stages. This type of analysis is readily incorporated into algorithms used to generate models with reference gene expression data.

As will be appreciated by those skilled in the art, the models are highly useful with even a small set of reference gene expression data and can become increasingly accurate with the inclusion of more reference data although the incremental increase in accuracy will likely diminish with each additional datum. The preparation of additional reference gene expression data using genes identified and disclosed herein for discriminating between different stages and/or grades of breast cancer is routine and may be readily performed by the skilled artisan to permit the generation of models as described above to predict the status of an unknown sample based upon the expression levels of those genes.

To determine the (increased or decreased) expression levels of genes in the practice of the present invention, any method known in the art may be utilized. In one preferred embodiment of the invention, expression based on detection of RNA which hybridizes to the genes identified and disclosed herein is used. This is readily performed by any RNA detection or amplification+detection method known or recognized as equivalent in the art such as, but not limited to, reverse transcription-PCR, the methods disclosed in U.S. patent application Ser. No. 10/062,857 entitled “Nucleic Acid Amplification” filed on Oct. 25, 2001 as well as U.S. Provisional Patent Applications 60/298,847 (filed Jun. 15, 2001) and 60/257,801 (filed Dec. 22, 2000), and methods to detect the presence, or absence, of RNA stabilizing or destabilizing sequences.

Alternatively, expression based on detection of DNA status may be used. Detection of the DNA of an identified gene as methylated or deleted may be used for genes that have decreased expression in correlation with a particular breast cancer stage and/or grade. This may be readily performed by PCR based methods known in the art, including, but not limited to, Q-PCR. Conversely, detection of the DNA of an identified gene as amplified may be used for genes that have increased expression in correlation with a particular breast cancer stage and/or grade. This may be readily performed by PCR based, fluorescent in situ hybridization (FISH) and chromosome in situ hybridization (CISH) methods known in the art.

Expression based on detection of a presence, increase, or decrease in protein levels or activity may also be used. Detection may be performed by any immunohistochemistry (IHC) based, blood based (especially for secreted proteins), antibody (including autoantibodies against the protein) based, ex foliate cell (from the cancer) based, mass spectroscopy based, and image (including used of labeled ligand) based method known in the art and recognized as appropriate for the detection of the protein. Antibody and image based methods are additionally useful for the localization of tumors after determination of cancer by use of cells obtained by a non-invasive procedure (such as ductal lavage or fine needle aspiration), where the source of the cancerous cells is not known. A labeled antibody or ligand may be used to localize the carcinoma(s) within a patient.

A preferred embodiment using a nucleic acid based assay to determine expression is by immobilization of one or more of the genes identified herein on a solid support, including, but not limited to, a solid substrate as an array or to beads or bead based technology as known in the art. Alternatively, solution based expression assays known in the art may also be used. The immobilized gene(s) may be in the form of polynucleotides that are unique or otherwise specific to the gene(s) such that the polynucleotide would be capable of hybridizing to a DNA or RNA corresponding to the gene(s). These polynucleotides may be the full length of the gene(s) or be short sequences of the genes (up to one nucleotide shorter than the full length sequence known in the art by deletion from the 5′ or 3′ end of the sequence) that are optionally minimally interrupted (such as by mismatches or inserted non-complementary basepairs) such that hybridization with a DNA or RNA corresponding to the gene(s) is not affected.

The immobilized gene(s) may be used to determine the state of nucleic acid samples prepared from sample breast cell(s) for which the pre-cancer or cancer status is not known or for confirmation of a status that is already assigned to the sample breast cell(s). Without limiting the invention, such a cell may be from a patient suspected of being afflicted with, or at risk of developing, breast cancer. The immobilized polynucleotide(s) need only be sufficient to specifically hybridize to the corresponding nucleic acid molecules derived from the sample. While even a single correlated gene sequence may to able to provide adequate accuracy in discriminating between two breast cancer cell stages and/or grades, two or more, three or more, four or more, five or more, six or more, seven or more, eight or more, nine or more, ten or more, or eleven or more of the genes identified herein may be used as a subset capable of discriminating may be used in combination to increase the accuracy of the method. The invention specifically contemplates the selection of more than one, two or more, three or more, four or more, five or more, six or more, seven or more, eight or more, nine or more, ten or more, or eleven or more of the genes disclosed in the tables and figures herein for use as a subset in the identification of whether an unknown or suspicious breast cancer sample is normal or is in one or more stages and/or grades of breast cancer. Optionally, the genes used will not include. CloneID 809507, which is also known as GenBank accession number AA454563, described as an EST with high similarity to CD63 but of unknown function.

In embodiments where only one or a few genes are to be analyzed, the nucleic acid derived from the sample breast cancer cell(s) may be preferentially amplified by use of appropriate primers such that only the genes to be analyzed are amplified to reduce contaminating background signals from other genes expressed in the breast cell. Alternatively, and where multiple genes are to be analyzed or where very few cells (or one cell) is used, the nucleic acid from the sample may be globally amplified before hybridization to the immobilized polynucleotides. Of course RNA, or the cDNA counterpart thereof may be directly labeled and used, without amplification, by methods known in the art.

The above assay embodiments may be used in a number of different ways to identify or detect the breast cancer stage and/or grade, if any, of a breast cancer cell sample from a patient. In many cases, this would reflect a secondary screen for the patient, who may have already undergone mammography or physical exam as a primary screen. If positive, the subsequent needle biopsy, ductal lavage, fine needle aspiration, or other analogous methods may provide the sample for use in the above assay embodiments. The present invention is particularly useful in combination with non-invasive protocols, such as ductal lavage or fine needle aspiration, to prepare a breast cell sample. The current analysis of ductal lavage samples is by cytological examination by a trained pathologist who classifies the samples in terms that are at least partly subjective: unsatisfactory (too few cells), benign (including fibrocystic change), atypical (or mild atypia), suspicious (or marked atypia), or malignant.

The present invention provides a more objective set of criteria, in the form of gene expression profiles of a discrete set of genes, to discriminate (or delineate) between meaningful stages and/or grades (or classes) of breast cancer cells. In particularly preferred embodiments of the invention, the assays are used to discriminate between the three grades (I, II, III) of carcinomas in situ as well as invasive carcinomas. With the use of alternative algorithms, such as neural networks, comparisons that discriminate between multiple (more than pairwise) classes may also be performed.

In one embodiment of the invention, the isolation and analysis of a breast cancer cell sample may be performed as follows:

-   -   (1) Ductal lavage or other non-invasive procedure is performed         on a patient to obtain a sample.     -   (2) Sample is prepared and coated onto a microscope slide. Note         that ductal lavage results in clusters of cells that are         cytologically examined as stated above.     -   (3) Pathologist or image analysis software scans the sample for         the presence of non-normal and/or atypical cells.     -   (4) If non-normal and/or atypical cells are observed, those         cells are harvested (e.g. by microdissection such as LCM).     -   (5) RNA is extracted from the harvested cells.     -   (6) RNA is purified, amplified, and labeled.     -   (7) Labeled nucleic acid is contacted with a microarray         containing polynucleotides of the genes identified herein as         correlated to discriminations between two or more stages of         breast cancer under hybridization conditions, then processed and         scanned to obtain a pattern of intensities of each spot         (relative to a control for general gene expression in cells)         which determine the level of expression of the gene(s) in the         cells.     -   (8) The pattern of intensities is analyzed by comparison to the         expression patterns of the genes in known samples of normal and         breast cancer cells (relative to the same control).

A specific example of the above method would be performing ductal lavage following a primary screen, observing and collecting non-normal and/or atypical cells for analysis. The comparison to known expression patterns, such as that made possible by a model generated by an algorithm (such as, but not limited to nearest neighbor type analysis, SVM, or neural networks) with reference gene expression data for the different breast cancer stages and/or grades, identifies the cells as being most likely grade III IDC.

Alternatively, the sample may permit the collection of both normal as well as non-normal and/or atypical cells for analysis. The gene expression patterns for each of these two samples will be compared to each other as well as the model and the normal versus individual abnormal comparisons therein based upon the reference data set. This approach can be significantly more powerful that the non-normal and/or atypical cells only approach because it utilizes significantly more information from the normal cells and the differences between normal and non-normal/atypical cells (in both the sample and reference data sets) to determine the status of the non-normal and/or atypical cells from the sample.

By appropriate selection of the genes used in the analysis, identification of the relative amounts of non-normal and/or atypical cells may also be possible, although in most clinical settings, the identification of the highest grade of breast cancer with confidence makes identification of lower grades less important. Stated differently, the identification of invasive cancer determines the clinical situation regardless of the presence of carcinoma in situ or hyperplastic cells, or the identification of carcinoma in situ makes determines the clinical situation regardless of the presence of hyperplastic cells. Similarly, the identification of a higher grade of cancer cells determines the clinical situation regardless of the presence of lower grades of cancer cells.

With use of the present invention, skilled physicians may prescribe treatments based on non-invasive samples that they would have prescribed for a patient which had previously received a diagnosis via a solid tissue biopsy.

The above discussion is also applicable where a palpable lesion is detected followed by fine needle aspiration or needle biopsy of cells from the breast. The cells are plated and reviewed by a pathologist or automated imaging system which selects cells for analysis as described above. This again provides a means of linking visual to molecular cytology and provides a less subjective means of identifying the physiological state of breast cancer cells without the need for invasive solid tissue biopsies.

The present invention may also be used, however, with solid tissue biopsies. For example, a solid biopsy may be collected and prepared for visualization followed by determination of expression of one or more genes identified herein to determine the stage of breast cancer, if any. One preferred means is by use of in situ hybridization with polynucleotide or protein identifying probe(s) for assaying expression of said gene(s).

In an alternative method, the solid tissue biopsy may be used to extract molecules followed by analysis for expression of one or more gene(s). This provides the possibility of leaving out the need for visualization and collection of only those cells suspected of being non-normal and/or atypical. This method may of course be modified such that only cells suspected of being non-normal and/or atypical are collected and used to extract molecules for analysis. This would require visualization and selection as an prerequisite to gene expression analysis.

In a further modification of the above, both normal cells and cells suspected of being non-normal and/or atypical are collected and used to extract molecules for analysis of gene expression. The approach, benefits and results are as described above using non-invasive sampling.

In a further alternative to all of the above, the gene(s) identified herein may be used as part of a simple PCR or array based assay simply to determine the presence of non-normal and/or atypical cells in a sample from a non-invasive sampling procedure. This is simple to perform and utilizes genes identified to be the best discriminators of normal versus abnormal cells without the need for any cytological examination. If no non-normal and/or atypical cells are identified, no cytological examination is necessary. If non-normal and/or atypical cells are identified, cytological examination follows, and a more comprehensive analysis, as described above, may follow.

The genes identified herein may be used to generate a model capable of predicting the breast canter stage and/or grade (if any) of an unknown breast cell sample based on the expression of the identified genes in the sample. Such a model may be generated by any of the algorithms described herein or otherwise known in the art as well as those recognized as equivalent in the art using gene(s) (and subsets thereof) disclosed herein for the identification of whether an unknown or suspicious breast cancer sample is normal or is in one or more stages and/or grades of breast cancer. The model provides a means for comparing expression profiles of gene(s) of the subset from the sample against the profiles of reference data used to build the model. The model can compare the sample profile against each of the reference profiles or against model defining delineations made based upon the reference profiles. Additionally, relative values from the sample profile may be used in comparison with the model or reference profiles.

In a preferred embodiment of the invention, breast cell samples identified as normal and non-normal and/or atypical from the same subject may be analyzed for their expression profiles of the genes used to generate the model. This provides an advantageous means of identifying the stage of the abnormal sample based on relative differences from the expression profile of the normal sample. These differences can then be used in comparison to differences between normal and individual abnormal reference data which was also used to generate the model.

The detection of gene expression from the samples may be by use of a single microarray able to assay gene expression from all pairwise comparisons disclosed herein for convenience and accuracy.

Other uses of the present invention include providing the ability to identify breast cancer cell samples as being those of a particular stage and/or grade of cancer for further research or study. This provides a particular advantage in many contexts requiring the identification of breast cancer stage and/or grade based on objective genetic or molecular criteria rather than cytological observation. It is of particular utility to distinguish different grades of a particular breast cancer stage for further study, research or characterization because no objective criteria for such delineation was previously available.

The materials for use in the methods of the present invention are ideally suited for preparation of kits produced in accordance with well known procedures. The invention thus provides kits comprising agents for the detection of expression of the disclosed genes for identifying breast cancer stage. Such kits optionally comprising the agent with an identifying description or label or instructions relating to their use in the methods of the present invention, is provided. Such a kit may comprise containers, each with one or more of the various reagents (typically in concentrated form) utilized in the methods, including, for example, pre-fabricated microarrays, buffers, the appropriate nucleotide triphosphates (e.g., dATP, dCTP, dGTP and dTTP; or rATP, rCTP, rGTP and UTP), reverse transcriptase, DNA polymerase, RNA polymerase, and one or more primer complexes of the present invention (e.g., appropriate length poly(T) or random primers linked to a promoter reactive with the RNA polymerase). A set of instructions will also typically be included.

The methods provided by the present invention may also be automated in whole or in part. All aspects of the present invention may also be practiced such that they consist essentially of a subset of the disclosed genes to the exclusion of material irrelevant to the identification of breast cancer stages in a cell containing sample.

Gene Expression Profiles of Pathological Stage and Histological Grade Progression of Human Breast Cancer

To identify gene expression changes that occur during breast cancer progression, isolation via LCM phenotypically of abnormal epithelium from ADH, DCIS and IDC and phenotypically normal epithelium (henceforth referred to as normal) from 36 breast cancer patients and 3 healthy mammoplasty reduction patients (FIG. 1A and Table 1) was performed. The resulting 300 independently microdissected samples were used to interrogate a microarray containing approximately 12,000 human genes. Genes showing significant differences in the pair-wise comparisons of normal vs. ADH, normal vs. DCIS and normal vs. IDC were selected by linear discriminant analysis, resulting in a total of 1940 unique genes for further exploration.

TABLE 1 Patient and tumor characteristics of clinical samples in this study Case ID Stages Microdissected Age ER PR HER2 Node^(a) 8 DCIS (III), IDC (III) 48 Pos Pos Pos Pos 14 N, DCIS (I), IDC (I) 44 Pos Pos ND Pos 22 ADH, DCIS (I) 44 ND ND ND Pos 25 DCIS (I), IDC (II) 81 Pos Neg ND ND 30 N, DCIS (III), IDC (III) 47 Neg Neg Neg Pos 41 N, DCIS (II), IDC (II) 55 Pos Pos ND Neg 43 N, DCIS (II), IDC (II) 53 Pos Neg Neg Pos 44 N, DCIS (III), IDC (III) 28 Pos Pos Neg Neg 45 N, DCIS (I) 36 Pos Neg Neg Neg ^(b)57 N, ADH, DCIS (I) 34 ND ND ND Neg 65 N, DCIS (III), IDC (III) 39 Pos Pos Neg Neg 78 MPR 46 79 N, ADH, DCIS (I), IDC (I) 54 Pos Pos Neg Pos 88 N, DCIS (III), IDC (III) 35 Pos Pos ND Pos 95 MPR 16 96 N, DCIS (III), IDC (III) 31 Neg Neg Neg Pos 97 DCIS (III), IDC (III) 79 Neg Neg Pos Pos 102 N, DCIS (I), IDC (I) 55 Pos Neg Neg Pos 112 N, DCIS (III), IDC (III) 31 Neg Pos Neg Pos 121 N, DCIS (II), IDC (II) 45 Pos Pos Pos Pos 130 N, DCIS (II), IDC (II) 54 Pos Pos Neg Pos 131 N, ADH, DCIS (II), IDC 37 Pos Pos Pos Pos (II) 133 N, DCIS (III), IDC (III) 44 Neg Neg Pos Pos 148 N, DCIS (II), IDC (II) 42 Pos Pos Neg Pos ^(b)152 N, DCIS (III) 55 ND ND ND Neg 153 N, IDC (I) 46 Pos Pos Pos Pos 169 N, DCIS (II), IDC (II) 34 Pos Pos Neg Pos 170 N, DCIS (II), IDC (II) 44 Pos Pos Pos-FISH Pos 173 N, DCIS (I), IDC (I) 52 Pos Pos Neg Neg 178 N, DCIS (III), IDC (III) 43 Pos Pos Pos Pos 179 N, DCIS (III), IDC (III) 37 Neg Neg Pos-FISH Pos 180 N, ADH, DCIS (I), IDC (I) 46 Pos Pos Neg Pos 183 N, DCIS (II) 46 ND ND ND Pos ^(b)191 N, ADH, DCIS (II) 43 ND ND ND 193 N, ADH, DCIS (I), IDC (I) 45 Pos Pos Neg Pos 198 N, DCIS (II), IDC (II) 30 Pos Pos Neg Neg ^(b)210 N, ADH, DCIS (I) 62 ND ND ND Neg ^(b)213 N, ADH 45 ND ND ND Neg 215 MPR 30 ^(a)Nodal status. Tumor grades indicated by roman numerals in parenthesis after the pathological stage of the specimen. Abbreviations used for pathological stages: N, normal; ADH, atypical ductal hyperplasia; DCIS, ductal carcinoma in situ; IDC, invasive ductal carcinoma; MPR, mammoplasty reduction. Abbreviations used for tumor marker status: ND, not determined; Pos, positive; Neg, negative; Pos-Fish, HER2-positivity by fluorescent in situ hybridization (FISH). ^(b)Individuals with pre-invasive breast cancer only.

One important advantage of LCM is the ability to procure both normal and diseased cell populations from the same biopsy. Therefore, the expression level of each gene in a disease state (ADH or DCIS or IDC) is represented as the ratio to the patient-matched normal, which highlights differences due to disease state as opposed to the genetic background of a particular patient. Unsupervised hierarchical clustering of the 1940 genes based on the resulting data across all samples reveals two main clusters (See FIG. 2a ). One cluster demonstrates increased expression in a majority of the diseased samples, and another cluster shows a relatively uniform decrease in expression across all samples. Importantly, most of these alterations (both increases and decreases) occur in the earliest stage of progression (ADH) and persist throughout later stages of DCIS and IDC. In addition, closer examination of this global view suggests that some of these genes increase their expression in DCIS/IDC of higher tumor grade. See Example II below.

Three example clusters of genes, further illustrate these points (FIG. 2b ). Cluster I consists of genes whose expression levels increase in ADH and persist in a majority of DCIS and IDC samples. The gene CRIP1 is especially prominent and thus may be a potential biomarker for the detection of breast cancer including the pre-malignant stage of ADH. The genes of Cluster I along with their I.M.A.G.E. Consortium CloneID number and descriptive identifiers are listed in Table 2.

TABLE 2 IMAGE CloneID Description 729975 MGEA5|meningioma expressed antigen 5 (hyaluronidase) 241043 Human clone 137308 mRNA, partial cds 1556859 ESTs, Weakly similar to I38022 hypothetical protein [H. sapiens] 1911343 RAB26|RAB26, member RAS oncogene family 589232 FLJ11506|hypothetical protein FLJ11506 138189 WFS1|Wolfram syndrome 1 (wolframin) 1323448 CRIP1|cysteine-rich protein 1 (intestinal) 488202 Homo sapiens cDNA FLJ31235 fis, clone KIDNE2004681, moderately similar to Mus musculus peroxisomal long chain acyl-CoA thioesterase Ib (Pte1b) gene 256619 HSD17B7|hydroxysteroid (17-beta) dehydrogenase 7 810063 GFER|growth factor, ervl (S. cerevisiae)-like (augmenter of liver regeneration) 824879 MGC11275|hypothetical protein MGC11275

Genes in cluster II display an expression pattern that correlate with tumor grade with the highest expression in grade III DCIS/IDC. Cluster II includes several genes important in the cell cycle (CENPA, HEC, UBE2C and PLK), and their elevated expression in grade III DCIS/IDC may reflect the higher proliferative index of high-grade tumors. The genes of Cluster II along with their I.M.A.G.E. Consortium CloneID number and descriptive identifiers are listed in Table 3.

TABLE 3 IMAGE CloneID Description 66406 ESTs, Highly similar to T47163 hypothetical protein DKFZp762E1312.1 [H. sapiens] 1517595 KIAA0175|likely ortholog of maternal embryonic leucine zipper kinase 2017415 CENPA|centromere protein A (17 kD) 345787 HEC|highly expressed in cancer, rich in leucine heptad repeats 504308 FLJ10540|hypothetical protein FLJ10540 769921 UBE2C|ubiquitin-conjugating enzyme E2C 128711 ANLN|anillin (Drosophila Scraps homolog), actin binding protein 744047 PLK|polo (Drosophia)-like kinase 128695 Homo sapiens, Similar to RIKEN cDNA 1810054O13 gene, clone IMAGE: 3845933, mRNA, partial cds

Genes in cluster III demonstrate decreased expression in all three pathological stages. The epithelium-specific transcription factor ELF5 is noteworthy since it maps to chromosome 11p13-15, a region subject to frequent loss of heterozygosity and rearrangement in multiple carcinoma including breast cancer (Zhou, J. et al. (1998a)). Therefore, loss of expression of ELF5 in ADH may be an important first step in the initiation of breast malignancy. Taken together, these results demonstrate that the normal to ADH transition is associated with extensive gene expression alterations and support the notion that ADH is a direct precursor to DCIS and IDC. The genes of Cluster III along with their I.M.A.G.E. Consortium CloneID number and descriptive identifiers are listed in Table 4.

TABLE 4 IMAGE CloneID Description 768007 CL683|weakly similar to glutathione peroxidase 2 877621 |nGAP-like protein 1570670 IL22RA2|class II cytokine receptor 1881774 KIAA1678|KIAA1678 1686766 |Rag D protein 505864 RGL|RalGDS-like gene 1569187 HS3ST4|heparan sulfate (glucosamine) 3-O-sulfotransferase 4 755881 AQP5|aquaporin 5 1864302 ELF5|E74-like factor 5 (ets domain transcription factor)

To gain further insight into the observation that different histological grades may be associated with distinct gene expression signatures (FIG. 2b , cluster II), two sets of genes were identified. Each comprised 100 genes correlating with grade I and grade III samples respectively using discriminant analysis. Again, to cancel out potential differences in the absolute levels of expression among individuals, gene expression values were expressed as ratios of ADH, DCIS or IDC to the corresponding normal. Unsupervised two-dimensional clustering revealed three major gene clusters (FIG. 3). One cluster of genes demonstrated decreased expression in all samples with subtle quantitative differences between grade I and grade III (green bar). A second cluster of genes (denoted as the grade III signature) shows markedly increased expression in grade III samples (red bar), whereas a third cluster (grade I signature) demonstrates increased expression primarily in grade I samples (blue bar). The genes of “green bar” genes along with their I.M.A.G.E. Consortium CloneID number, chromosomal location and descriptive identifiers (if known) are listed in Table 5.

TABLE 5 IMAGE Chromosomal Clone ID location Description 471196 2q37 ITM3|integral membrane protein 3 796904 6q24-q25 PLAGL1|pleiomorphic adenoma gene-like 1 32493 2q31.1 ITGA6|“integrin, alpha 6” 1534700 11q21 KIAA0830|KIAA0830 protein 712139 2q37.2 ARL7|ADP-ribosylation factor-like 7 291478 1p36 RUNX3|runt-related transcription factor 3 150897 19p13.1 B3GNT3|“UDP-GlcNAc:betaGal beta-1,3-N-acetylglucosaminyltransferase 3” 1653105 3p14-p12 TSP50|testes-specific protease 50 665384 16 KIAA1609|KIAA1609 protein 842818 16q23-q24 KARS|lysyl-tRNA synthetase 37671 18q11.2 FLJ21610|hypothetical protein FLJ21610 773301 16q22.1 CDH3|“cadherin 3, type 1, P-cadherin (placental)” 503671 6 Homo sapiens cDNA FLJ14368 fis, clone HEMBA1001122 3172883 11 ESTs, Weakly similar to S24195 dopamine receptor D4 [H. sapiens] 684890 16p12.1 FLJ20274|hypothetical protein FLJ20274 593840 17q11.2 DKFZP564K1964|DKFZP564K1964 protein 121454 17p13.1 ALOX12|arachidonate 12-lipoxygenase 197913 1p34.2 SFPQ|splicing factor proline/glutamine rich (polypyrimidine tract-binding protein- associated) 43090 20q13.12 H-L(3)MBT|lethal (3) malignant brain tumor I(3)mbt protein (Drosophila) homolog 814826 2 ESTs 1635062 12q13.13 DKFZP586A011|DKFZP586A011 protein 814815 1601845 7q22-q31.1 CAPRI|Ca2+-promoted Ras inactivator 190059 19p13.3 GNG7|“guanine nucleotide binding protein (G protein), gamma 7” 277044 19q13.32 KIAA1183|KIAA1183 protein 1592530 3p21.31 IP6K2|mammalian inositol hexakisphosphate kinase 2 431231 11q13 EFEMP2|EGF-containing fibulin-like extracellular matrix protein 2 267254 17 ESTs, Highly similar to LOX2_HUMAN ARACHIDONATE 12-LIPOXYGENASE [H. sapiens] 43679 10 ESTs 295572 12q24.21 KIAA0682|KIAA0682 gene product 46129 12q13.1 HDAC7A|histone deacetylase 7A 1569077 6 EST 138242 1 ESTs, Moderately similar to MAS2_human mannan-binding lectin serine protease 2 precursor [H. sapiens] 417637 4p16 KIAA1276|KIAA1276 protein 248631 3p21.2-p21.1 AMT|aminomethyltransferase (glycine cleavage system protein T) 1553530 2 KIAA0788|KIAA0788 protein 307029 1883169 5p15.32 FLJ20303|hypothetical protein FLJ20303 345764 3p23 SATB1|special AT-rich sequence binding protein 1 (binds to nuclear matrix/scaffold- associating DNA's) 703964 11q23 INPPL1|inositol polyphosphate phosphatase-like 1 70349 Xq13.1 MLLT7|“myeloid/lymphoid or mixed-lineage leukemia (trithorax (Drosophila) homolog); translocated to, 7” 1868349 15q11.2-q21.3 PLA2G4B|“phospholipase A2, group IVB (cytosolic)” 126466 1p34.1 KIAA0467|KIAA0467 protein 1631682 1p32 PPIE|peptidylprolyl isomerase E (cyclophilin E) 172783 19 ZNF358|zinc finger protein 358 1566877 11q13 C11orf2|chromosome 11 open reading frame2 1630990 3p21.3-p21.2 RPL29|ribosomal protein L29 283124 19 Homo sapiens, clone IMAGE: 3917549, mRNA, partial cds 126415 10 Homo sapiens mRNA; cDNA DKFZp566H0124 (from clone DKFZp566H0124) 344168 10q23 POLL|“polymerase (DNA directed), lambda” 823634 10 ESTs 325583 EST 810741 17p13.2 GABARAP|GABA(A) receptor-associated protein 511831 3 MGC12936|hypothetical protein MGC12936 180561 1p13.3 GSTM1|glutathione S-transferase M1 206217 11p11.2 NR1H3|“nuclear receptor subfamily 1, group H, member 3” 108667 22q12.2 SF3A1|“splicing factor 3a, subunit 1, 120 kD” 839796 12p13.31 LOC51147|candidate tumor suppressor p33 ING1 homolog 502518 3p21 LAMB2|“laminin, beta 2 (laminin S)” 810981 22q13 FLJ20699|hypothetical protein FLJ20699 1635059 9 Homo sapiens, clone MGC: 16638 IMAGE: 4121964, mRNA, complete cds 767176 17p13.1 TNFSF13|“tumor necrosis factor (ligand) superfamily, member 13” 810358 17p13-p11 ACADVL|“acyl-Coenzyme A dehydrogenase, very long chain” 2757710 10p11.2 ZNF37A|zinc finger protein 37a (KOX 21) 1652259 7q31.3 LKR/SDH|lysine-ketoglutarate reductase/saccharopine dehydrogenase

The genes of “red bar” genes along with their I.M.A.G.E. Consortium CloneID number, chromosomal location and descriptive-identifiers (if known) are listed in Table 6.

TABLE 6 IMAGE Chromosomal Clone ID location Description 293727 22q13.2 MGC861|hypothetical protein MGC861 843121 6p22.1-p21.2 CLIC1|chloride intracellular channel 1 839682 12q22 UBE2N|ubiquitin-conjugating enzyme E2N (homologous to yeast UBC13) 815501 19p13.3 MGC2721|hypothetical protein MGC2721 1587847 2q21 MCM6|“minichromosome maintenance deficient (mis5, S. pombe) 6” 1416055 8 KIAA0165|“extra spindle poles, S. cerevisiae, homolog of” 2018131 12p13.2-p13.1 RACGAP1|Rac GTPase activating protein 1 1476053 15q15.1 RAD51|RAD51 (S. cerevisiae) homolog (E coli RecA homolog) 869375 15q26.1 IDH2|“isocitrate dehydrogenase 2 (NADP+), mitochondrial” 951241 15q13.3 ANKT|nucleolar protein ANKT 743810 12p13 MGC2577|hypothetical protein MGC2577 292936 1p34.3 FLJ10468|hypothetical protein FLJ10468 66406 2 ESTs, Highly similar to T47163 hypothetical protein DKFZp762E1312.1 [H. sapiens] 1517595 9p11.2 KIAA0175|likely ortholog of maternal embryonic leucine zipper kinase 2017415 2p24-p21 CENPA|centromere protein A (17 kD) 345787 18p11.31 HEC|“highly expressed in cancer, rich in leucine heptad repeats” 504308 10cen-q26.11 FLJ10540|hypothetical protein FLJ10540 769921 20q13.12 UBE2C|ubiquitin-conjugating enzyme E2C 128711 7p15-p14 ANLN|“anillin (Drosophila Scraps homolog), actin binding protein” 744047 16p12.3 PLK|polo (Drosophia)-like kinase 564981 18 Homo sapiens, Similar to RIKEN cDNA 2810433K01 gene, clone MGC: 10200 IMAGE: 3909951, mRNA, complete cds 259950 8q23 CML66|chronic myelogenous leukemia tumor antigen 66 825606 10q24.1 KNSL1|kinesin-like 1 814270 4q27 PMSCL1|polymyositis/scleroderma autoantigen 1 (75 kD) 785368 8p21-p12 TOPK|PDZ-binding kinase; T-cell originated protein kinase 209066 20q13.2-q13.3 STK15|serine/threonine kinase 15 739450 1q21.2 LASS2|“longevity assurance (LAG1, S. cerevisiae) homolog 2” 1702742 16q24.3 SLC7A5|“solute carrier family 7 (cationic amino acid transporter, y+ system), member 5” 1631634 9q34.11 MGC3038|“hypothetical protein similar to actin related protein 2/3 complex, subunit 5” 725454 9q22 CKS2|CDC28 protein kinase 2 825470 17q21-q22 TOP2A|topoisomerase (DNA) II alpha (170 kD) 796469 1q32.1 HSPC150|HSPC150 protein similar to ubiquitin-conjugating enzyme 705064 4p16.3 TACC3|“transforming, acidic coiled-coil containing protein 3” 471568 17q25 HN1|hematological and neurological expressed 1 742707 7 ESTs, Weakly similar to MUC2_HUMAN MUCIN 2 PRECURSOR [H. sapiens] 624667 9q34.13 LOC51117|CGI-92 protein 1422338 2p25-p24 RRM2|ribonucleotide reductase M2 polypeptide 700792 14q22 CDKN3|cyclin-dependent kinase inhibitor 3 (CDK2-associated dual specificity phosphatase) 280375 8p22 PRO2000|PRO2000 protein 122241 1p34.2 PSMB2|“proteasome (prosome, macropain) subunit, beta type, 2” 2309073 2q33-q34 FZD5|frizzled (Drosophila) homolog 5 2322367 2p14-p13 RTN4|reticulon 4 796694 17q25 BIRC5|baculoviral IAP repeat-containing 5 (survivin) 74677 Homo sapiens, Similar to RIKEN cDNA A430107J06 gene, clone MGC: 21416 IMAGE: 4452699, mRNA, complete cds 824524 17q21.32 UGTREL1|UDP-galactose transporter related 825282 DKFZP586L0724|DKFZP586L0724 protein 824962 17q23.1-q23.3 KPNA2|“karyopherin alpha 2 (RAG cohort 1, importin alpha 1)” 42831 11q11-q12 NTKL|N-terminal kinase-like 814054 1q24-25 KIAA0040|KIAA0040 gene product 2054635 20q13.33 PSMA7|“proteasome (prosome, macropain) subunit, alpha type, 7” 210862 17q24-17q25 ACOX1|“acyl-Coenzyme A oxidase 1, palmitoyl” 897997 Xp11.22-p11.21 SMC1L1|“SMC1 (structural maintenance of chromosomes 1, yeast)-like 1” 769890 14q13.1 NP|nucleoside phosphorylase 756595 1q21 S100A10|“S100 calcium-binding protein A10 (annexin II ligand, calpactin I, light polypeptide (p11))” 951233 2q35 PSMB3|“proteasome (prosome, macropain) subunit, beta type, 3” 529827 Xp22.31 SYAP1|reserved 1660666 Xp21.1 CA5B|“carbonic anhydrase VB, mitochondrial” 1696757 13q22.2 KIAA1165|hypothetical protein KIAA1165 361922 1p34 ZMPSTE24|“zinc metalloproteinase, STE24 (yeast, homolog)” 823598 PSMD12|“proteasome (prosome, macropain) 26S subunit, non-ATPase, 12” 772220 3q21.2 PDIR|for protein disulfide isomerase-related 703707 8q12.1 ASPH|aspartate beta-hydroxylase 78869 20q13.33 GP110|“cell membrane glycoprotein, 110000M(r) (surface antigen)” 1474424 17 Homo sapiens cDNA FLJ31911 fis, clone NT2RP7004751 1947647 17q23.3 LOC51651|CGI-147 protein 897609 12q23.2 FLJ10074|hypothetical protein FLJ10074 753378 4q34.1 FLJ22649|hypothetical protein FLJ22649 similar to signal peptidase SPC22/23 124331 16 CPSF5|“cleavage and polyadenylation specific factor 5, 25 kD subunit” 327506 15 Homo sapiens mRNA full length insert cDNA clone EUROIMAGE 327506 345538 9q21-q22 CTSL|cathepsin L 753320 8q13.3 FLJ20533|hypothetical protein FLJ20533 823907 8q12.2 FLJ10511|hypothetical protein FLJ10511 149355 8q13.1 TRAM|translocating chain-associating membrane protein 347373 8q13.3 TCEB1|“transcription elongation factor B (SIII), polypeptide 1 (15 kD, elongin C)” 2028949 17q21.31 PRO1855|hypothetical protein PRO1855 624627 2p25-p24 RRM2|ribonucleotide reductase M2 polypeptide 731023 9q34 WDR5|WD repeat domain 5 786067 20p13 CDC25B|cell division cycle 25B 878330 3 Homo sapiens cDNA: FLJ22044 fis, clone HEP09141 1631132 11q12.1 PHT2|peptide transporter 3 756442 7q11.2 POR|P450 (cytochrome) oxidoreductase 823930 7q22.1 ARPC1A|“actin related protein 2/3 complex, subunit 1A (41 kD)” 268946 2 Homo sapiens cDNA FLJ31861 fis, clone NT2RP7001319 1914863 2p13.3-p13.1 DYSF|“dysferlin, limb girdle muscular dystrophy 2B (autosomal recessive)” 789012 3p25-p24 FBLN2|fibulin 2 781047 2q14 BUB1|budding uninhibited by benzimidazoles 1 (yeast homolog) 753428 8 Homo sapiens, Similar to RIKEN cDNA 1110014B07 gene, clone MGC: 20766 IMAGE: 4586039, mRNA, complete cds

The genes of “blue bar” genes along with their I.M.A.G.E. Consortium CloneID number, chromosomal location and descriptive identifiers (if known) are listed in Table 7.

TABLE 7 IMAGE Chromosomal Clone ID location Description 286378 19q13.4 ZNF135|zinc finger protein 135 (clone pHZ-17) 854763 2q31.1 MGC20702|hypothetical protein MGC20702 344959 4p16.2 HSA250839|gene for serine/threonine protein kinase 278222 18 Homo sapiens, clone MGC: 10083 IMAGE: 3897118, mRNA, complete cds 1679977 18 Homo sapiens, clone MGC: 10083 IMAGE: 3897118, mRNA, complete cds 504959 11 Homo sapiens mRNA; cDNA DKFZp586G0321 (from clone DKFZp586G0321) 342181 18q21.3 BCL2|B-cell CLL/lymphoma 2 502988 19p13.3-p13.2 ZNF20|zinc finger protein 20 (KOX 13) 590310 2 Homo sapiens, clone MGC: 17393 IMAGE: 3914851, mRNA, complete cds 186301 11 Homo sapiens cDNA FLJ12924 fis, clone NT2RP2004709 357120 16 Homo sapiens, clone IMAGE: 3538007, mRNA, partial cds 203003 16p13.3 NME4|“non-metastatic cells 4, protein expressed in” 725649 14q11.2 NFATC4|“nuclear factor of activated T-cells, cytoplasmic, calcineurin-dependent 4” 2014373 2q11.2 HNK-1ST|HNK-1 sulfotransferase 183440 22q13.33 ARSA|arylsulfatase A 2014856 1q25.3 HLALS|“major histocompatibility complex, class I-like sequence” 256619 10p11.2 HSD17B7|hydroxysteroid (17-beta) dehydrogenase 7 768570 1q21.2 FLJ11280|hypothetical protein FLJ11280 2975668 11p13 RAG2|recombination activating gene 2 278430 2q23.3 KIF5C|kinesin family member 5C 1558233 3 ESTs 627248 5q23.2 SBBI31|SBBI31 protein 1517171 10p15-p14 IL2RA|“interleukin 2 receptor, alpha” 1492468 1p32.3 KIAA0452|DEME-6 protein 292770 1 Homo sapiens, clone IMAGE: 3627860, mRNA, partial cds 1456701 1q21 BCL9|B-cell CLL/lymphoma 9 743146 18p11.21 FLJ23403|hypothetical protein FLJ23403 1557637 5 ESTs 1583198 5 ESTs, Weakly similar to S65824 reverse transcriptase homolog [H. sapiens] 741891 6p21.3 RAB2L|“RAB2, member RAS oncogene family-like” 179572 1 Homo sapiens cDNA FLJ14227 fis, clone NT2RP3004095 1569902 16p11.2 KIAA0556|KIAA0556 protein 127646 18 ESTs, Weakly similar to T00365 hypothetical protein KIAA0670 [H. sapiens] 782688 1p35.1 P28|“dynein, axonemal, light intermediate polypeptide” 1883630 15 KIAA1547|KIAA1547 protein 725340 4p16.3 TETRAN|tetracycline transporter-like protein 726890 10q24.2 MGC4643|hypothetical protein MGC4643 82322 2p23.3 RBSK|ribokinase 839382 9 Homo sapiens, Similar to RIKEN cDNA 1700017I11 gene, clone MGC: 26847 IMAGE: 4821517, mRNA, complete cds 49630 3p14.3 CACNA1D|“calcium channel, voltage-dependent, L type, alpha 1D subunit” 32050 2 Homo sapiens mRNA; cDNA DKFZp586P1124 (from clone DKFZp586P1124) 110226 TNFRSF10C|“tumor necrosis factor receptor superfamily, member 10c, decoy without an intracellular domain” 1932725 1q32.1 ZNF281|zinc finger protein 281 279720 11 Homo sapiens, Similar to RIKEN cDNA 1700008D07 gene, clone MGC: 9830 IMAGE: 3863323, mRNA, complete cds 1733262 3p21.3 BLu|BLu protein 197903 1 ESTs, Moderately similar to unnamed protein product [H. sapiens] 1556859 17 ESTs, Weakly similar to I38022 hypothetical protein [H. sapiens] 726699 16 Homo sapiens, clone MGC: 9889 IMAGE: 3868330, mRNA, complete cds

Most striking is the existence of reciprocal gradients in the intensities of these two signatures from grade I to grade III with most grade II lesions exhibiting both signatures to varying degrees (e.g., cases 130, 169, 198). Interestingly, some grade II lesions show an expression pattern that is most similar to either grade I or grade III lesions (case 41 and 43, respectively), and some grade III samples also express the grade I signature (e.g., cases 65, 88 and 112). Histological grade is an important characteristic of breast cancer with proven utility in patient prognostication and treatment (Fitzgibbons, P. L. et al.). For example, tumors of grade III are more likely to recur and are more likely to respond to chemotherapy than those of grade I (Page, D. L. et al. (2001)). However, the current tumor grading system relies mainly on histomorphological criteria, which, although highly successful in differentiating grade I from grade III tumors, are inadequate to score grade II tumors consistently (Dalton, L. W. et al.). This difficulty may be explained by the existence of a transcriptional continuum from grade I to grade III as we observed here. Therefore, a gene expression-based molecular grading system may allow greater precision in classifying breast cancer and provide greater insight into the state of progression of a particular tumor.

An expanded set of 250 genes that display increased expression in Grade I samples in comparison to Grade III samples are identified in Table 8 by use of their I.M.A.G.E. Consortium CloneID numbers along with their chromosomal location and descriptive identifiers (if known) and relative weights.

TABLE 8 IMAGE Chromosome Clone ID Weight Location Description 344959 1.451333 4p16.2 HSA250839 | gene for serine/threonine protein kinase 504959 1.28687 11 Homo sapiens mRNA; cDNA DKFZp586G0321 (from clone DKFZp586G0321) 814815 1.2414 743146 1.221818 18p11.21 FLJ23403 | hypothetical protein FLJ23403 417637 1.208243 4p16 KIAA1276 | KIAA1276 protein 502988 1.133964 19p13.3-p13.2 ZNF20 | zinc finger protein 20 (KOX 13) 1679977 1.131337 18 Homo sapiens, clone MGC: 10083 IMAGE: 3897118, mRNA, complete cds 342181 1.12098 18q21.3 BCL2 | B-cell CLL/lymphoma 2 1932725 1.11409 1q32.1 ZNF281 | zinc finger protein 281 70349 1.110469 Xq13.1 MLLT7 | myeloid/lymphoid or mixed-lineage leukemia (trithorax (Drosophila) homolog); translocated to, 7 180561 1.077508 1p13.3 GSTM1 | glutathione S-transferase M1 186301 1.068369 11 Homo sapiens cDNA FLJ12924 fis, clone NT2RP2004709 278222 1.065646 18 Homo sapiens, clone MGC: 10083 IMAGE: 3897118, mRNA, complete cds 357120 1.062902 16 Homo sapiens, clone IMAGE: 3538007, mRNA, partial cds 248631 1.04971 3p21.2-p21.1 AMT | aminomethyltransferase (glycine cleavage system protein T) 43090 1.021857 20q13.12 H-L(3)MBT | lethal (3) malignant brain tumor l(3)mbt protein (Drosophila) homolog 1631682 1.021091 1p32 PPIE | peptidylprolyl isomerase E (cyclophilin E) 767176 1.003495 17p13.1 TNFSF13 | tumor necrosis factor (ligand) superfamily, member 13 325583 1.00279 EST 1883630 0.979795 15 KIAA1547 | KIAA1547 protein 32050 0.979642 2 Homo sapiens mRNA; cDNA DKFZp586P1124 (from clone DKFZp586P1124) 502518 0.962484 3p21 LAMB2 | laminin, beta 2 (laminin S) 126415 0.957069 10 Homo sapiens mRNA; cDNA DKFZp566H0124 (from clone DKFZp566H0124) 82322 0.946458 2p23.3 RBSK | ribokinase 2975668 0.936737 11p13 RAG2 | recombination activating gene 2 1558233 0.931636 3 ESTs 256619 0.928002 10p11.2 HSD17B7 | hydroxysteroid (17-beta) dehydrogenase 7 206217 0.92794 11p11.2 NR1H3 | nuclear receptor subfamily 1, group H, member 3 726890 0.926526 10q24.2 MGC4643 | hypothetical protein MGC4643 2014373 0.906969 2q11.2 HNK-1ST | HNK-1 sulfotransferase 283124 0.89695 19 Homo sapiens, clone IMAGE: 3917549, mRNA, partial cds 741891 0.887613 6p21.3 RAB2L | RAB2, member RAS oncogene family-like 49630 0.885374 3p14.3 CACNA1D | calcium channel, voltage-dependent, L type, alpha 1D subunit 1592530 0.871817 3p21.31 IP6K2 | mammalian inositol hexakisphosphate kinase 2 277044 0.868338 19q13.32 KIAA1183 | KIAA1183 protein 1566877 0.867336 11q13 C11orf2 | chromosome 11 open reading frame2 839796 0.867221 12p13.31 LOC51147 | candidate tumor suppressor p33 ING1 homolog 279720 0.864865 11 Homo sapiens, Similar to RIKEN cDNA 1700008D07 gene, clone MGC: 9830 IMAGE: 3863323, mRNA, complete cds 511831 0.854961 3 MGC12936 | hypothetical protein MGC12936 2014856 0.849103 1q25.3 HLALS | major histocompatibility complex, class I-like sequence 1652259 0.845966 7q31.3 LKR/SDH | lysine-ketoglutarate reductase/saccharopine dehydrogenase 172783 0.844046 19 ZNF358 | zinc finger protein 358 267254 0.838823 17 ESTs, Highly similar to LOX2_HUMAN ARACHIDONATE 12-LIPOXYGENASE [H. sapiens] 725340 0.826253 4p16.3 TETRAN | tetracycline transporter-like protein 593840 0.82327 17q11.2 DKFZP564K1964 | DKFZP564K1964 protein 179572 0.819502 1 Homo sapiens cDNA FLJ14227 fis, clone NT2RP3004095 854763 0.818371 2q31.1 MGC20702 | hypothetical protein MGC20702 286378 0.818288 19q13.4 ZNF135 | zinc finger protein 135 (clone pHZ-17) 1733262 0.815457 3p21.3 BLu | BLu protein 1517171 0.812481 10p15-p14 IL2RA | interleukin 2 receptor, alpha 814826 0.807648 2 ESTs 126466 0.797965 1p34.1 KIAA0467 | KIAA0467 protein 110226 0.796159 TNFRSF10C | tumor necrosis factor receptor superfamily, member 10c, decoy without an intracellular domain 344168 0.795755 10q23 POLL | polymerase (DNA directed), lambda 108667 0.79402 22q12.2 SF3A1 | splicing factor 3a, subunit 1, 120 kD 295572 0.792031 12q24.21 KIAA0682 | KIAA0682 gene product 823634 0.789164 10 ESTs 138242 0.787686 1 ESTs, Moderately similar to MAS2_HUMAN MANNAN-BINDING LECTIN SERINE PROTEASE 2 PRECURSOR [H. sapiens] 197903 0.785879 1 ESTs, Moderately similar to unnamed protein product [H. sapiens] 292770 0.784314 1 Homo sapiens, clone IMAGE: 3627860, mRNA, partial cds 810981 0.784118 22q13 FLJ20699 | hypothetical protein FLJ20699 197913 0.777546 1p34.2 SFPQ | splicing factor proline/glutamine rich (polypyrimidine tract-binding protein- associated) 190059 0.77474 19p13.3 GNG7 | guanine nucleotide binding protein (G protein), gamma 7 782688 0.77051 1p35.1 P28 | dynein, axonemal, light intermediate polypeptide 121454 0.76967 17p13.1 ALOX12 | arachidonate 12-lipoxygenase 1569902 0.764217 16p11.2 KIAA0556 | KIAA0556 protein 726699 0.760736 16 Homo sapiens, clone MGC: 9889 IMAGE: 3868330, mRNA, complete cds 1601845 0.759847 7q22-q31.1 CAPRI | Ca2+-promoted Ras inactivator 703964 0.759625 11q23 INPPL1 | inositol polyphosphate phosphatase-like 1 183440 0.757148 22q13.33 ARSA | arylsulfatase A 431231 0.756281 11q13 EFEMP2 | EGF-containing fibulin-like extracellular matrix protein 2 810358 0.750312 17p13-p11 ACADVL | acyl-Coenzyme A dehydrogenase, very long chain 1583198 0.749857 5 ESTs, Weakly similar to S65824 reverse transcriptase homolog [H. sapiens] 1630990 0.748442 3p21.3-p21.2 RPL29 | ribosomal protein L29 1868349 0.746257 15q11.2-q21.3 PLA2G4B | phospholipase A2, group IVB (cytosolic) 627248 0.744679 5q23.2 SBBI31 | SBBI31 protein 127646 0.743672 18 ESTs, Weakly similar to T00365 hypothetical protein KIAA0670 [H. sapiens] 1635059 0.739062 9 Homo sapiens, clone MGC: 16638 IMAGE: 4121964, mRNA, complete cds 1456701 0.732349 1q21 BCL9 | B-cell CLL/lymphoma 9 345764 0.72889 3p23 SATB1 | special AT-rich sequence binding protein 1 (binds to nuclear matrix/scaffold- associating DNA's) 278430 0.728595 2q23.3 KIF5C | kinesin family member 5C 1492468 0.72665 1p32.3 KIAA0452 | DEME-6 protein 590310 0.725531 2 Homo sapiens, clone MGC: 17393 IMAGE: 3914851, mRNA, complete cds 768570 0.720983 1q21.2 FLJ11280 | hypothetical protein FLJ11280 1883169 0.716948 5p15.32 FLJ20303 | hypothetical protein FLJ20303 1635062 0.716142 12q13.13 DKFZP586A011 | DKFZP586A011 protein 2757710 0.715294 10p11.2 ZNF37A | zinc finger protein 37a (KOX 21) 810741 0.709032 17p13.2 GABARAP | GABA(A) receptor-associated protein 1569077 0.708429 6 EST 1653105 0.708359 3p14-p12 TSP50 | testes-specific protease 50 1553530 0.707954 2 KIAA0788 | KIAA0788 protein 43679 0.707235 10 ESTs 725649 0.706826 14q11.2 NFATC4 | nuclear factor of activated T-cells, cytoplasmic, calcineurin-dependent 4 684890 0.705934 16p12.1 FLJ20274 | hypothetical protein FLJ20274 1556859 0.702746 17 ESTs, Weakly similar to I38022 hypothetical protein [H. sapiens] 1557637 0.698307 5 ESTs 203003 0.697573 16p13.3 NME4 | non-metastatic cells 4, protein expressed in 46129 0.694321 12q13.1 HDAC7A | histone deacetylase 7A 839382 0.693177 9 Homo sapiens, Similar to RIKEN cDNA 1700017I11 gene, clone MGC: 26847 IMAGE: 4821517, mRNA, complete cds 307029 0.690207 184022 0.689767 11p15 APBB1 | amyloid beta (A4) precursor protein-binding, family B, member 1 (Fe65) 745077 0.681153 19 Homo sapiens mRNA; cDNA DKFZp566J2324 (from clone DKFZp566J2324); partial cds 769600 0.68017 5p15.2-p13.1 UNG2 | uracil-DNA glycosylase 2 280776 0.677821 15 MGC5139 | hypothetical protein MGC5139 810947 0.674861 16p13.11 NUDE1 | LIS1-interacting protein NUDE1, rat homolog 824879 0.674702 16p13.3 MGC11275 | hypothetical protein MGC11275 454503 0.669502 12 Homo sapiens, clone IMAGE: 3346451, mRNA, partial cds 811920 0.658971 9p13 IL11RA | interleukin 11 receptor, alpha 1636360 0.658963 15q21.1-q21.2 FLJ14957 | hypothetical protein FLJ14957 2502722 0.658146 11q23 LOH11CR2A | loss of heterozygosity, 11, chromosomal region 2, gene A 1609372 0.657294 14q11.2 RIPK3 | receptor-interacting serine-threonine kinase 3 346977 0.655725 3p24.3 KIAA0210 | KIAA0210 gene product 293569 0.653314 1q25 C1orf21 | chromosome 1 open reading frame 21 1635307 0.651746 12 Homo sapiens, clone IMAGE: 3833472, mRNA 240505 0.65172 14q11.2 KIAA0323 | KIAA0323 protein 52724 0.648958 FLJ20241 | hypothetical protein FLJ20241 120138 0.648579 10q21.1 JDP1 | J domain containing protein 1 74070 0.648244 1q21.2 ENSA | endosulfine alpha 186626 0.644915 6 ESTs, Weakly similar to CYP4_HUMAN 40 KDA PEPTIDYL-PROLYL CIS-TRANS ISOMERASE [H. sapiens] 296679 0.644155 5 Homo sapiens clone TCCCTA00151 mRNA sequence 2119838 0.64368 11q25 ADAMTS8 | a disintegrin-like and metalloprotease (reprolysin type) with thrombospondin type 1 motif, 8 813488 0.643211 1q32.1 LOC51235 | hypothetical protein 742094 0.639857 14q32.12 FLJ20950 | hypothetical protein FLJ20950 705274 0.638802 2q37.2 DGKD | diacylglycerol kinase, delta (130 kD) 826285 0.633833 Homo sapiens cDNA FLJ32001 fis, clone NT2RP7009373 358217 0.631361 Xq26.1 GPC4 | glypican 4 796723 0.629143 Homo sapiens clone CDABP0014 mRNA sequence 529843 0.628435 19 ESTs 262251 0.627736 16p13 CLCN7 | chloride channel 7 490449 0.623346 5q31 RAD50 | RAD50 (S. cerevisiae) homolog 788334 0.622909 11p15.5-p15.4 MRPL23 | mitochondrial ribosomal protein L23 1909935 0.62043 8 ESTs 250883 0.61921 3p21 UBE1L | ubiquitin-activating enzyme E1-like 1707667 0.618023 17 Homo sapiens cDNA FLJ31065 fis, clone HSYRA2001142 68103 0.617869 12 MLC1SA | myosin light chain 1 slow a 773381 0.617263 19q13.33 NAPA | N-ethylmaleimide-sensitive factor attachment protein, alpha 1559596 0.616776 11 ESTs, Highly similar to AF175283 1 zinc metalloendopeptidase [H. sapiens] 825296 0.616769 1q42.11-q42.3 LDLC | low density lipoprotein receptor defect C complementing 866866 0.616211 3p21.3 RASSF1 | Ras association (RalGDS/AF-6) domain family 1 490668 0.613699 3 Homo sapiens, clone IMAGE: 4182947, mRNA 824052 0.613652 6p21.3 C6orf1 | chromosome 6 open reading frame 1 505243 0.612671 12p11 ITPR2 | inositol 1,4,5-triphosphate receptor, type 2 1911343 0.612387 16p13.3 RAB26 | RAB26, member RAS oncogene family 1637296 0.60612 10q22-q23 RPS24 | ribosomal protein S24 753252 0.604292 17q21.31 MGC4251 | hypothetical protein MGC4251 1518890 0.602612 11q13.2-q13.3 MTL5 | metallothionein-like 5, testis-specific (tesmin) 234522 0.601183 1q21.3 KIAA1535 | KIAA1535 protein 52419 0.598962 9q13-q21 X123 | Friedreich ataxia region gene X123 278483 0.598475 18p11.32 TYMS | thymidylate synthetase 877664 0.598243 20 FLJ14987 | hypothetical protein FLJ14987 826622 0.594938 16p13.12 KIAA0430 | KIAA0430 gene product 701112 0.591773 3p25 XPC | xeroderma pigmentosum, complementation group C 1859625 0.591377 8q24 BAI1 | brain-specific angiogenesis inhibitor 1 812975 0.586956 9p23 KIAA0172 | KIAA0172 protein 214068 0.585918 10p15 GATA3 | GATA-binding protein 3 1587863 0.581689 3p23-p22 ACAA1 | acetyl-Coenzyme A acyltransferase 1 (peroxisomal 3-oxoacyl-Coenzyme A thiolase) 1518402 0.576275 17q11.1 KIAA1361 | KIAA1361 protein 796996 0.57565 Xq13.1-q13.3 IGBP1 | immunoglobulin (CD79A) binding protein 1 1323448 0.575218 7q11.23 CRIP1 | cysteine-rich protein 1 (intestinal) 2388571 0.574109 19p13.1-q12 AKAP8 | A kinase (PRKA) anchor protein 8 75078 0.573276 12 ESTs 1604642 0.572299 6 Homo sapiens cDNA FLJ32724 fis, clone TESTI2000951 66532 0.572179 20q13.2-q13.3 EDN3 | endothelin 3 2273445 0.571917 20q11.2 GHRH | growth hormone releasing hormone 346643 0.567626 10 ESTs 595297 0.563887 1q21.3 SNAPAP | SNARE associated protein snapin 971399 0.561448 12cen-q21 SYT1 | synaptotagmin I 897550 0.561065 17q21.2 MGC2744 | hypothetical protein MGC2744 215000 0.560663 3p22 VIPR1 | vasoactive intestinal peptide receptor 1 155896 0.560564 11cen-q12.1 LOC51035 | ORF 1700429 0.56053 10q26 GFRA1 | GDNF family receptor alpha 1 277463 0.560068 18p11.2 C18orf1 | chromosome 18 open reading frame 1 1587710 0.556854 17p13.1-17p12 PER1 | period (Drosophila) homolog 1 565849 0.55621 1q32.1 C3IP1 | kelch-like protein C3IP1 126851 0.555748 10q22.1 FLJ11160 | hypothetical protein FLJ11160 2413337 0.554359 11q23.2-q24.2 SORL1 | sortilin-related receptor, L(DLR class) A repeats-containing 824753 0.554027 13 FLJ22624 | hypothetical protein FLJ22624 50471 0.553058 11 Homo sapiens cDNA FLJ14242 fis, clone OVARC1000678 33500 0.552872 Homo sapiens clone 23556 mRNA sequence 752547 0.551916 15 Homo sapiens mRNA; cDNA DKFZp586G1520 (from clone DKFZp586G1520) 83358 0.550166 ESTs 2096306 0.55013 8q24.3 ARC | activity-regulated cytoskeleton-associated protein 196189 0.548574 18q23 CYB5 | cytochrome b-5 2018808 0.546276 11q14 PRCP | prolylcarboxypeptidase (angiotensinase C) 1500542 0.544517 16p13.3 RGS11 | regulator of G-protein signalling 11 470061 0.544311 3q25 SIAH2 | seven in absentia (Drosophila) homolog 2 1762111 0.543871 5p14-p13 NPR3 | natriuretic peptide receptor C/guanylate cyclase C (atrionatriuretic peptide receptor C) 2116188 0.543472 17q21 HDAC5 | histone deacetylase 5 826668 0.542351 6q21 KIAA0274 | KIAA0274 gene product 26736 0.540638 20 Homo sapiens cDNA FLJ30872 fis, clone FEBRA2004293 669379 0.540325 7 Homo sapiens, clone IMAGE: 3463399, mRNA, partial cds 221776 0.536594 14 ESTs, Weakly similar to T20410 hypothetical protein E02A10.2 - Caenorhabditis elegans [C. elegans] 264632 0.535737 19 ESTs 741790 0.53497 2p13.3 FLJ20080 | hypothetical protein FLJ20080 1626087 0.53252 3p21.31 DKFZP434A236 | DKFZP434A236 protein 812033 0.532407 2q35-q37 GPC1 | glypican 1 950574 0.531092 17q25 H3F3B | H3 histone, family 3B (H3.3B) 284022 0.531011 8p23 ARHGEF10 | Rho guanine nucleotide exchange factor (GEF) 10 35828 0.528716 5q23 DTR | diphtheria toxin receptor (heparin-binding epidermal growth factor-like growth factor) 2284619 0.528522 19q13.4 ZNF132 | zinc finger protein 132 (clone pHZ-12) 681992 0.528384 7 Homo sapiens cDNA FLJ13384 fis, clone PLACE1001062, highly similar to Homo sapiens mRNA for lysine-ketoglutarate reductase/saccharopine dehydrogenase 43933 0.52806 Xp11.4-p11.3 MAOA | monoamine oxidase A 785538 0.527955 Homo sapiens cDNA FLJ32293 fis, clone PROST2001739 343760 0.526569 6q13-15 SH3BGRL2 | SH3 domain binding glutamic acid-rich protein like 2 785571 0.525679 10 DNAJL1 | hypothetical protein similar to mouse Dnajl1 809507 0.525406 16p13.3 FLJ20568 | hypothetical protein FLJ20568 1895664 0.524227 15q26.1 PRO2198 | hypothetical protein PRO2198 823661 0.521218 14 Homo sapiens cDNA FLJ31768 fis, clone NT2RI2007891, moderately similar to DMR-N9 PROTEIN 842980 0.519909 22q12.2 DRG1 | developmentally regulated GTP-binding protein 1 126419 0.517789 1q21-q22 NIT1 | nitrilase 1 1926023 0.516851 7 ESTs, Weakly similar to T42727 proliferation potential-related protein - mouse [M. musculus] 132857 0.516382 17 Homo sapiens mRNA; cDNA DKFZp586N1323 (from clone DKFZp586N1323) 855586 0.515352 5q31 NR3C1 | nuclear receptor subfamily 3, group C, member 1 810331 0.515056 1q24 QSCN6 | quiescin Q6 265103 0.512718 1p36 MMEL2 | membrane metallo-endopeptidase-like 2 1521361 0.511233 8p21.2 KIAA0717 | KIAA0717 protein 432072 0.508774 18q23 NFATC1 | nuclear factor of activated T-cells, cytoplasmic, calcineurin-dependent 1 2069602 0.506115 16q24.3 MC1R | melanocortin 1 receptor (alpha melanocyte stimulating hormone receptor) 283173 0.505655 4 Homo sapiens PAC clone RP1-130H16 from 22q12.1-qter 1404841 0.501049 19q13.4 ZNF175 | zinc finger protein 175 1871116 0.500004 2 Homo sapiens mRNA; cDNA DKFZp434C1714 (from clone DKFZp434C1714); partial cds 758365 0.4988 12q13-q15 OS4 | conserved gene amplified in osteosarcoma 1641894 0.498542 10 ESTs 1492147 0.498131 Xq13.1 RPS4X | ribosomal protein S4, X-linked 1558642 0.497736 2q37.3 MLPH | melanophilin 1641245 0.497723 18q21.1 LOC51320 | hypothetical protein 1635649 0.497647 20p13 CDS2 | CDP-diacylglycerol synthase (phosphatidate cytidylyltransferase) 2 414999 0.496855 17q21 ETV4 | ets variant gene 4 (E1A enhancer-binding protein, E1AF) 1535957 0.496325 5p15.3 SEC6 | similar to S. cerevisiae Sec6p and R. norvegicus rsec6 774082 0.495883 12q22-q23 ASCL1 | achaete-scute complex (Drosophila) homolog-like 1 811013 0.494705 1p13.3 AMPD2 | adenosine monophosphate deaminase 2 (isoform L) 809998 0.493372 1p21 AMY2A | amylase, alpha 2A; pancreatic 2018084 0.48899 2q24.3 SPAK | Ste-20 related kinase 161373 0.485425 7q11-q22 PMS2L4 | postmeiotic segregation increased 2-like 4 178137 0.485162 4q25 RPL34 | ribosomal protein L34 75886 0.484926 4 ESTs, Weakly similar to E54024 protein kinase [H. sapiens] 429387 0.484053 7p15.3 CHN2 | chimerin (chimaerin) 2 742977 0.481369 7p13 DKFZP761I2123 | KIAA1886 protein 240637 0.480946 1p33-p32.1 MGC8974 | hypothetical protein MGC8974 838366 0.480888 1p36.1-p35 HMGCL | 3-hydroxymethyl-3-methylglutaryl-Coenzyme A lyase (hydroxymethylglutaricaciduria) 796181 0.480102 13q34 GAS6 | growth arrest-specific 6 23776 0.479727 4p15.31 QDPR | quinoid dihydropteridine reductase 1909433 0.478064 17 Homo sapiens cDNA FLJ30754 fis, clone FEBRA2000438 2160920 0.477446 1p13 PHTF1 | putative homeodomain transcription factor 1 1500536 0.475933 12pter-p13.31 MDS028 | uncharacterized hematopoietic stem/progenitor cells protein MDS028 294537 0.474189 2q37.3 RAB17 | RAB17, member RAS oncogene family 784085 0.469813 6q25-q26 TUSP | tubby super-family protein 239877 0.469171 5q31 HDAC3 | histone deacetylase 3 626861 0.468844 11p15 EIF4G2 | eukaryotic translation initiation factor 4 gamma, 2 741977 0.466816 6p21.3 BF | B-factor, properdin

Some of the genes within the tumor grade VIII signatures have been previously reported to be associated with breast cancer. Within the grade I signature, two genes, BCL2 and TNFRSF10C, are inhibitors of apoptosis. Various reports in the literature link BCL2 expression to ER-positive, low-grade tumors (van Slooten, H. J. et al.). TNFRSF10C is a decoy receptor (DcR1) for TRAIL, an apoptosis-inducing cytokine of the tumor necrosis factor (TNF) family (Sheridan, J. P. et al.). Without being bound by theory, presence of DcR1 on the surface of breast cancer cells would be expected to block signaling through the cell death receptors activated by TRAIL, thus inhibiting apoptosis.

Similarly, an expanded set of 250 genes that display increased expression in Grade III samples in comparison to Grade I samples are identified in Table 9 by use of their I.M.A.G.E. Consortium CloneID numbers along with their chromosomal location and descriptive identifiers (if known) and relative weights (which are expressed with a negative sign solely due to the relative comparison).

TABLE 9 IMAGE Chromosome Clone ID Weight Location Description 769921 −1.53568 20q13.12 UBE2C | ubiquitin-conjugating enzyme E2C 951241 −1.33815 15q13.3 ANKT | nucleolar protein ANKT 1517595 −1.3332 9p11.2 KIAA0175 | likely ortholog of maternal embryonic leucine zipper kinase 1474424 −1.32072 17 Homo sapiens cDNA FLJ31911 fis, clone NT2RP7004751 2309073 −1.29533 2q33-q34 FZD5 | frizzled (Drosophila) homolog 5 796469 −1.27516 1q32.1 HSPC150 | HSPC150 protein similar to ubiquitin-conjugating enzyme 823598 −1.26568 PSMD12 | proteasome (prosome, macropain) 26S subunit, non-ATPase, 12 700792 −1.25232 14q22 CDKN3 | cyclin-dependent kinase inhibitor 3 (CDK2-associated dual specificity phosphatase) 2018131 −1.23217 12p13.2-p13.1 RACGAP1 | Rac GTPase activating protein 1 292936 −1.20973 1p34.3 FLJ10468 | hypothetical protein FLJ10468 1422338 −1.20922 2p25-p24 RRM2 | ribonucleotide reductase M2 polypeptide 504308 −1.18743 10cen-q26.11 FLJ10540 | hypothetical protein FLJ10540 796694 −1.16444 17q25 BIRC5 | baculoviral IAP repeat-containing 5 (survivin) 869375 −1.15363 15q26.1 IDH2 | isocitrate dehydrogenase 2 (NADP+), mitochondrial 814270 −1.14538 4q27 PMSCL1 | polymyositis/scleroderma autoantigen 1 (75 kD) 42831 −1.12878 11q11-q12 NTKL | N-terminal kinase-like 1476053 −1.10462 15q15.1 RAD51 | RAD51 (S. cerevisiae) homolog (E coli RecA homolog) 32493 −1.10275 2q31.1 ITGA6 | integrin, alpha 6 149355 −1.10225 8q13.1 TRAM | translocating chain-associating membrane protein 824962 −1.09918 17q23.1-q23.3 KPNA2 | karyopherin alpha 2 (RAG cohort 1, importin alpha 1) 1702742 −1.09644 16q24.3 SLC7A5 | solute carrier family 7 (cationic amino acid transporter, y+ system), member 5 824524 −1.07854 17q21.32 UGTREL1 | UDP-galactose transporter related 128711 −1.07401 7p15-p14 ANLN | anillin (Drosophila Scraps homolog), actin binding protein 843121 −1.06508 6p22.1-p21.2 CLIC1 | chloride intracellular channel 1 2017415 −1.06388 2p24-p21 CENPA | centromere protein A (17 kD) 753378 −1.0364 4q34.1 FLJ22649 | hypothetical protein FLJ22649 similar to signal peptidase SPC22/23 825470 −1.03507 17q21-q22 TOP2A | topoisomerase (DNA) II alpha (170 kD) 705064 −1.02376 4p16.3 TACC3 | transforming, acidic coiled-coil containing protein 3 2054635 −1.02042 20q13.33 PSMA7 | proteasome (prosome, macropain) subunit, alpha type, 7 781047 −1.0153 2q14 BUB1 | budding uninhibited by benzimidazoles 1 (yeast homolog) 1534700 −1.01343 11q21 KIAA0830 | KIAA0830 protein 1587847 −1.01171 2q21 MCM6 | minichromosome maintenance deficient (mis5, S. pombe) 6 743810 −1.0099 12p13 MGC2577 | hypothetical protein MGC2577 897609 −0.99379 12q23.2 FLJ10074 | hypothetical protein FLJ10074 66406 −0.98421 2 ESTs, Highly similar to T47163 hypothetical protein DKFZp762E1312.1 [H. sapiens] 1631634 −0.98233 9q34.11 MGC3038 | hypothetical protein similar to actin related protein 2/3 complex, subunit 5 624627 −0.96436 2p25-p24 RRM2 | ribonucleotide reductase M2 polypeptide 814054 −0.95575 1q24-25 KIAA0040 | KIAA0040 gene product 773301 −0.91294 16q22.1 CDH3 | cadherin 3, type 1, P-cadherin (placental) 1416055 −0.91005 8 KIAA0165 | extra spindle poles, S. cerevisiae, homolog of 345787 −0.89554 18p11.31 HEC | highly expressed in cancer, rich in leucine heptad repeats 624667 −0.88376 9q34.13 LOC51117 | CGI-92 protein 786067 −0.87714 20p13 CDC25B | cell division cycle 25B 785368 −0.87699 8p21-p12 TOPK | PDZ-binding kinase; T-cell originated protein kinase 564981 −0.85513 18 Homo sapiens, Similar to RIKEN cDNA 2810433K01 gene, clone MGC: 10200 IMAGE: 3909951, mRNA, complete cds 753320 −0.85505 8q13.3 FLJ20533 | hypothetical protein FLJ20533 529827 −0.85016 Xp22.31 SYAP1 | reserved 122241 −0.84842 1p34.2 PSMB2 | proteasome (prosome, macropain) subunit, beta type, 2 712139 −0.84823 2q37.2 ARL7 | ADP-ribosylation factor-like 7 259950 −0.83947 8q23 CML66 | chronic myelogenous leukemia tumor antigen 66 772220 −0.83895 3q21.2 PDIR | for protein disulfide isomerase-related 124331 −0.83664 16 CPSF5 | cleavage and polyadenylation specific factor 5, 25 kD subunit 842818 −0.83338 16q23-q24 KARS | lysyl-tRNA synthetase 150897 −0.82922 19p13.1 B3GNT3 | UDP-GlcNAc:betaGal beta-1,3-N-acetylglucosaminyltransferase 3 823930 −0.82876 7q22.1 ARPC1A | actin related protein 2/3 complex, subunit 1A (41 kD) 210862 −0.82312 17q24-17q25 ACOX1 | acyl-Coenzyme A oxidase 1, palmitoyl 731023 −0.82276 9q34 WDR5 | WD repeat domain 5 665384 −0.82232 16 KIAA1609 | KIAA1609 protein 815501 −0.82108 19p13.3 MGC2721 | hypothetical protein MGC2721 769890 −0.81864 14q13.1 NP | nucleoside phosphorylase 209066 −0.81121 20q13.2-q13.3 STK15 | serine/threonine kinase 15 471568 −0.81026 17q25 HN1 | hematological and neurological expressed 1 725454 −0.80701 9q22 CKS2 | CDC28 protein kinase 2 951233 −0.80178 2q35 PSMB3 | proteasome (prosome, macropain) subunit, beta type, 3 268946 −0.79976 2 Homo sapiens cDNA FLJ31861 fis, clone NT2RP7001319 2028949 −0.78651 17q21.31 PRO1855 | hypothetical protein PRO1855 1914863 −0.78621 2p13.3-p13.1 DYSF | dysferlin, limb girdle muscular dystrophy 2B (autosomal recessive) 744047 −0.77737 16p12.3 PLK | polo (Drosophila)-like kinase 703707 −0.77579 8q12.1 ASPH | aspartate beta-hydroxylase 78869 −0.76948 20q13.33 GP110 | cell membrane glycoprotein, 110000M(r) (surface antigen) 742707 −0.7686 7 ESTs, Weakly similar to MUC2_HUMAN MUCIN 2 PRECURSOR [H. sapiens] 825606 −0.75817 10q24.1 KNSL1 | kinesin-like 1 361922 −0.7559 1p34 ZMPSTE24 | zinc metalloproteinase, STE24 (yeast, homolog) 756595 −0.75094 1q21 S100A10 | S100 calcium-binding protein A10 (annexin II ligand, calpactin I, light polypeptide (p11)) 756442 −0.7508 7q11.2 POR | P450 (cytochrome) oxidoreductase 823907 −0.74968 8q12.2 FLJ10511 | hypothetical protein FLJ10511 471196 −0.74806 2q37 ITM3 | integral membrane protein 3 753428 −0.74668 8 Homo sapiens, Similar to RIKEN cDNA 1110014B07 gene, clone MGC: 20766 IMAGE: 4586039, mRNA, complete cds 739450 −0.74247 1q21.2 LASS2 | longevity assurance (LAG1, S. cerevisiae) homolog 2 1696757 −0.73849 13q22.2 KIAA1165 | hypothetical protein KIAA1165 293727 −0.73213 22q13.2 MGC861 | hypothetical protein MGC861 839682 −0.731 12q22 UBE2N | ubiquitin-conjugating enzyme E2N (homologous to yeast UBC13) 1631132 −0.73053 11q12.1 PHT2 | peptide transporter 3 327506 −0.72966 15 Homo sapiens mRNA full length insert cDNA clone EUROIMAGE 327506 1660666 −0.72774 Xp21.1 CA5B | carbonic anhydrase VB, mitochondrial 280375 −0.72588 8p22 PRO2000 | PRO2000 protein 796904 −0.71939 6q24-q25 PLAGL1 | pleiomorphic adenoma gene-like 1 503671 −0.71201 6 Homo sapiens cDNA FLJ14368 fis, clone HEMBA1001122 74677 −0.71194 Homo sapiens, Similar to RIKEN cDNA A430107J06 gene, clone MGC: 21416 IMAGE: 4452699, mRNA, complete cds 291478 −0.71127 1p36 RUNX3 | runt-related transcription factor 3 825282 −0.7096 DKFZP586L0724 | DKFZP586L0724 protein 878330 −0.70859 3 Homo sapiens cDNA: FLJ22044 fis, clone HEP09141 37671 −0.70374 18q11.2 FLJ21610 | hypothetical protein FLJ21610 789012 −0.7019 3p25-p24 FBLN2 | fibulin 2 347373 −0.70161 8q13.3 TCEB1 | transcription elongation factor B (SIII), polypeptide 1 (15 kD, elongin C) 2322367 −0.69997 2p14-p13 RTN4 | reticulon 4 897997 −0.69961 Xp11.22-p11.21 SMC1L1 | SMC1 (structural maintenance of chromosomes 1, yeast)-like 1 345538 −0.69527 9q21-q22 CTSL | cathepsin L 1947647 −0.69371 17q23.3 LOC51651 | CGI-147 protein 3172883 −0.69164 11 ESTs, Weakly similar to S24195 dopamine receptor D4 [H. sapiens] 1035796 −0.68832 1 ESTs, Weakly similar to T33068 hypothetical protein C35E7.9 - Caenorhabditis elegans [C. elegans] 746163 −0.67918 8 ESTs, Weakly similar to ALU1_HUMAN ALU SUBFAMILY J SEQUENCE CONTAMINATION WARNING ENTRY [H. sapiens] 810711 −0.67743 10q23-q24 SCD | stearoyl-CoA desaturase (delta-9-desaturase) 462926 −0.67573 1q32.2-q41 NEK2 | NIMA (never in mitosis gene a)-related kinase 2 1614140 −0.67368 15q11.2-q22.33 LOC51285 | Ris 124781 −0.66984 8q24.1 SQLE | squalene epoxidase 1642496 −0.66639 2p24.1 MGC11266 | hypothetical protein MGC11266 113300 −0.66053 9q22.32 TRIM14 | tripartite motif-containing 14 2014034 −0.65845 2p12 MTHFD2 | methylene tetrahydrofolate dehydrogenase (NAD+ dependent), methenyltetrahydrofolate cyclohydrolase 1946448 −0.65464 7q31.1 CAV2 | caveolin 2 1635352 −0.65164 4q12 TPARL | TPA regulated locus 753400 −0.64918 3q27.1 BAF53A | BAF53 1605426 −0.64391 4q12 FLJ13352 | hypothetical protein FLJ13352 565319 −0.64374 8 MAL2 | mal, T-cell differentiation protein 2 489755 −0.64095 10q26.3 ADAM12 | a disintegrin and metalloproteinase domain 12 (meltrin alpha) 1916461 −0.63993 22 Homo sapiens, clone IMAGE: 3605655, mRNA 359887 −0.63379 1q32.1 TIM17 | translocase of inner mitochondrial membrane 17 homolog A (yeast) 629944 −0.63018 18q12 MYO5B | myosin VB 150314 −0.62891 6q13 LYPLA1 | lysophospholipase I 770355 −0.62829 21q22.3 LSS | lanosterol synthase (2,3-oxidosqualene-lanosterol cyclase) 489594 −0.6245 Xq22.2 FLJ11565 | hypothetical protein FLJ11565 212640 −0.6219 Xq28 ARHGAP4 | Rho GTPase activating protein 4 30170 −0.62007 4q34 CASP3 | caspase 3, apoptosis-related cysteine protease 51773 −0.61957 7p15-p14 MGC3077 | hypothetical protein MGC3077 490777 −0.61906 1858892 −0.61695 Xp22.13 MGC4825 | hypothetical protein MGC4825 358456 −0.61552 7p11.2 SEC61G | Sec61 gamma 840894 −0.61414 12q24.2 COX6A1 | cytochrome c oxidase subunit VIa polypeptide 1 241348 −0.61157 PCL1 | prenylcysteine lyase 1505038 −0.61123 8q22.2 FLJ20171 | hypothetical protein FLJ20171 144880 −0.60976 19p13.3 LOC56932 | hypothetical protein from EUROIMAGE 1759349 454896 −0.60575 16q11.1-q11.2 DNAJA2 | DnaJ (Hsp40) homolog, subfamily A, member 2 753236 −0.60461 6 ESTs, Weakly similar to S71512 hypothetical protein T2 - mouse [M. musculus] 266218 −0.60106 418159 −0.60025 22q13.1 SYNGR1 | synaptogyrin 1 208718 −0.59862 9q12-q21.2 ANXA1 | annexin A1 781097 −0.59718 11q13 RTN3 | reticulon 3 469383 −0.59434 8q21 C8orf1 | chromosome 8 open reading frame 1 725152 −0.59375 11q11 DKFZp762A227 | hypothetical protein DKFZp762A227 845363 −0.59313 17q21.3 NME1 | non-metastatic cells 1, protein (NM23A) expressed in 1460110 −0.59206 14q11.2 PSMB5 | proteasome (prosome, macropain) subunit, beta type, 5 769959 −0.5913 13q34 COL4A2 | collagen, type IV, alpha 2 796527 −0.59108 7q34 DKFZp761N0624 | hypothetical protein DKFZp761N0624 108425 −0.59009 1 ESTs, Weakly similar to JC5314 CDC28/cdc2-like kinase associating arginine- serine cyclophilin [H. sapiens] 32231 −0.58516 FLJ12442 | hypothetical protein FLJ12442 502690 −0.58445 3q21.3-q25.2 RPN1 | ribophorin I 135221 −0.58203 4p16 S100P | S100 calcium-binding protein P 897813 −0.58167 17p11.1 PAIP1 | polyadenylate binding protein-interacting protein 1 824352 −0.58119 9q31.2 RAD23B | RAD23 (S. cerevisiae) homolog B 897751 −0.58057 17q23 TLK2 | tousled-like kinase 2 343607 −0.57727 15q14-q24.3 LOC55829 | AD-015 protein 51899 −0.5772 16q24.1 KIAA0513 | KIAA0513 gene product 726645 −0.57716 16q23 CLECSF1 | C-type (calcium dependent, carbohydrate-recognition domain) lectin, superfamily member 1 (cartilage-derived) 1591264 −0.57558 11p15.5-p15.4 TALDO1 | transaldolase 1 290841 −0.57171 6p21.3 H2BFA | H2B histone family, member A 486626 −0.57063 8 Homo sapiens, clone IMAGE: 4332938, mRNA 221846 −0.56769 14q24.3-q31 CHES1 | checkpoint suppressor 1 772913 −0.56751 5 Homo sapiens cDNA FLJ31951 fis, clone NT2RP7007177, weakly similar to Homo sapiens multiple membrane spanning receptor TRC8 mRNA 1686766 −0.56178 6q15-q16 RAGD | Rag D protein 37708 −0.56053 16q24.3 MGC3101 | hypothetical protein MGC3101 825740 −0.56021 2q32.1 DKFZP434J1813 | DKFZp434J1813 protein 741139 −0.56009 20q13.1 EYA2 | eyes absent (Drosophila) homolog 2 754293 −0.55369 2p12 C2orf6 | chromosome 2 open reading frame 6 83363 −0.55322 6q24-q25 PCMT1 | protein-L-isoaspartate (D-aspartate) O-methyltransferase 686552 −0.55207 1q42.13 GOLPH1 | golgi phosphoprotein 1 950429 −0.54962 12q KIAA1708 | KIAA1708 protein 813419 −0.54843 Xp11.2 HADH2 | hydroxyacyl-Coenzyme A dehydrogenase, type II 2043167 −0.54694 10q25.2-q26.2 BAG3 | BCL2-associated athanogene 3 701115 −0.54546 6 PRO2013 | hypothetical protein PRO2013 795498 −0.54391 15q26.1 HS1-2 | putative transmembrane protein 965223 −0.54333 17q23.2-q25.3 TK1 | thymidine kinase 1, soluble 377191 −0.53874 8p22-q22.1 LOC51123 | HSPC038 protein 233679 −0.53609 2p23.3 FLJ22362 | hypothetical protein FLJ22362 590759 −0.53571 4q32-q34 SC4MOL | sterol-C4-methyl oxidase-like 358083 −0.53534 3q29 KIAA0226 | KIAA0226 gene product 810612 −0.53335 1q21 S100A11 | S100 calcium-binding protein A11 (calgizzarin) 220395 −0.52987 2p22.3 FLJ23293 | likely ortholog of mouse ADP-ribosylation-like factor 6 interacting protein 2 280699 −0.52812 7 UCC1 | upregulated in colorectal cancer gene 1 2016775 −0.52687 16p12 GPRC5B | G protein-coupled receptor, family C, group 5, member B 470124 −0.52331 5p13.2 RAD1 | RAD1 (S. pombe) homolog 154707 −0.51926 2p23-p21 MPV17 | MpV17 transgene, murine homolog, glomerulosclerosis 785933 −0.51884 Xp21.1 SRPX | sushi-repeat-containing protein, X chromosome 2062825 −0.51819 20q11.23 KIAA0964 | KIAA0964 protein 2009491 −0.51791 4q22.1-q23 LOC51191 | cyclin-E binding protein 1 1534493 −0.51765 8 ESTs 150003 −0.5167 8q22.2 FLJ13187 | phafin 2 950600 −0.51409 1 Homo sapiens mRNA; cDNA DKFZp586C1019 (from clone DKFZp586C1019) 1455394 −0.51333 7p15.2 HCS | cytochrome c 811918 −0.51318 20p12.1 KIAA0952 | KIAA0952 protein 415191 −0.51 2p25.3 KIAA0161 | KIAA0161 gene product 32927 −0.50974 8q24.3 FBXL6 | f-box and leucine-rich repeat protein 6 1845744 −0.50818 325160 −0.50752 3q13.13 NP25 | neuronal protein 812048 −0.50542 20pter-p12 PRNP | prion protein (p27-30) (Creutzfeld-Jakob disease, Gerstmann- Strausler-Scheinker syndrome, fatal familial insomnia) 84161 −0.50451 DKFZP434F195 | DKFZP434F195 protein 897806 −0.50236 14q21-q24 HIF1A | hypoxia-inducible factor 1, alpha subunit (basic helix-loop-helix transcription factor) 814378 −0.50026 19q13.1 SPINT2 | serine protease inhibitor, Kunitz type, 2 188335 −0.49789 EMR2 | egf-like module containing, mucin-like, hormone receptor-like sequence 2 1585492 −0.49501 9 ESTs 133213 −0.49332 11q21 FUT4 | fucosyltransferase 4 (alpha (1,3) fucosyltransferase, myeloid-specific) 73009 −0.49156 5 Homo sapiens, clone MGC: 9628 IMAGE: 3913311, mRNA, complete cds 785707 −0.49031 15q26.1 PRC1 | protein regulator of cytokinesis 1 84464 −0.49025 1q42.12 FLJ12806 | hypothetical protein FLJ12806 770066 −0.48965 11q25 KIAA0056 | KIAA0056 protein 41208 −0.48944 8p21 BMP1 | bone morphogenetic protein 1 1698036 −0.48904 20q13.2 UBE2V1 | ubiquitin-conjugating enzyme E2 variant 1 1435862 −0.4889 Xp22.32 MIC2 | antigen identified by monoclonal antibodies 12E7, F21 and O13 768452 −0.48449 21 Homo sapiens EST from clone 491476, full insert 824426 −0.48229 7q22.1 PDAP1 | PDGFA associated protein 1 768561 −0.48129 17q11.2-q21.1 SCYA2 | small inducible cytokine A2 (monocyte chemotactic protein 1, homologous to mouse Sig-je) 377275 −0.48092 11q22-q23 TRIM29 | tripartite motif-containing 29 470128 −0.48 15q21-q22 MYO1E | myosin IE 809901 −0.47984 9q21-q22 COL15A1 | collagen, type XV, alpha 1 50772 −0.47983 7p14-p13 MGC3251 | hypothetical protein MGC3251 1843843 −0.47902 12q14.1 SRGAP1 | KIAA1304 protein 823940 −0.47897 17q21 TOB1 | transducer of ERBB2, 1 564492 −0.47749 11p11.12 MTCH2 | mitochondrial carrier homolog 2 290101 −0.47734 X ESTs 263894 −0.47704 16p12.1 QPRT | quinolinate phosphoribosyltransferase (nicotinate-nucleotide pyrophosphorylase (carboxylating)) 202901 −0.47699 9q34.1 VAV2 | vav 2 oncogene 1607229 −0.47609 6q22-q23 TPD52L1 | tumor protein D52-like 1 812050 −0.47584 8q24 TRC8 | patched related protein translocated in renal cancer 1637756 −0.47545 1p36.3-p36.2 ENO1 | enolase 1, (alpha) 813410 −0.47231 8q22.3 POLR2K | polymerase (RNA) II (DNA directed) polypeptide K (7.0 kD) 358162 −0.47197 11q13.1 HSU79266 | protein predicted by clone 23627 2062238 −0.47184 2q37.1 PSMD1 | proteasome (prosome, macropain) 26S subunit, non-ATPase, 1 753215 −0.47119 7q21 GNAI1 | guanine nucleotide binding protein (G protein), alpha inhibiting activity polypeptide 1 739126 −0.46952 8q24.3 TSTA3 | tissue specific transplantation antigen P35B 1917941 −0.46918 7p13 H2AV | histone H2A.F/Z variant 111362 −0.46893 20q11.2 OSBPL2 | oxysterol-binding protein-like 2 1456348 −0.46742 9p24.1-p23 SAS | N-acetylneuraminic acid phosphate synthase; sialic acid synthase 263716 −0.46636 21q22.3 COL6A1 | collagen, type VI, alpha 1 810156 −0.46594 2 DTYMK | deoxythymidylate kinase (thymidylate kinase) 115443 −0.46519 HSPC216 | hypothetical protein 32299 −0.46427 18p11.2 IMPA2 | inositol(myo)-1(or 4)-monophosphatase 2 1434897 −0.46024 2q14-q32 COL5A2 | collagen, type V, alpha 2 2028916 −0.45905 10 Homo sapiens mRNA for Hmob33 protein, 3′ untranslated region 2020898 −0.45878 7q22 PLOD3 | procollagen-lysine, 2-oxoglutarate 5-dioxygenase 3 487797 −0.45837 1p22.1 DR1 | down-regulator of transcription 1, TBP-binding (negative cofactor 2) 284734 −0.45795 6q21-q22 WASF1 | WAS protein family, member 1 79520 −0.45632 8q12.1 RAB2 | RAB2, member RAS oncogene family 812977 −0.45368 12 Homo sapiens mesenchymal stem cell protein DSC96 mRNA, partial cds 810899 −0.45368 ESTs 428163 −0.45286 3 ESTs, Weakly similar to NAH6_HUMAN SODIUM/HYDROGEN EXCHANGER 6 [H. sapiens] 613056 −0.45261 11p13 RCN1 | reticulocalbin 1, EF-hand calcium binding domain 741474 −0.45249 19q13.1 GPI | glucose phosphate isomerase 768989 −0.45147 14 Homo sapiens cDNA FLJ12874 fis, clone NT2RP2003769 754702 −0.45087 2p25.1-p24.1 KIAA0846 | KIAA0846 protein 246800 −0.45055 7p13 FLJ10803 | hypothetical protein FLJ10803 246304 −0.4503 21q21.1 BTG3 | BTG family, member 3

The grade III signature contains genes known to be involved in cell cycle control (CKS2, CDC25B, MCM6), chromosomal segregation (STK15, CENPA and TACC3), and DNA recombination and repair (RAD51, UBE2N, TOP2A, RRM2). In particular, CDC25B, potential oncogene, transforms murine diploid fibroblasts into high-grade tumors (Galaktionov, K. et al.). STK15, a centrosomal protein kinase, is frequently amplified in breast cancer, and its quantitative expression levels positively correlate with tumor grade (Zhou, H. et al. (1998b)). RAD51 has recently been shown to interact with the tumor suppressor BRCA1 (Chen, J. J., et al. (1999)), and its expression also positively correlates with tumor grade in breast cancer (Maacke, H. et al.). It has not been previously known or suspected, however, whether the expression of these genes would be capable of differentiating grade III breast cancer cells from grade I breast cancer cells. Without being bound by theory, abnormal expression of the genes associated with DNA recombination and repair and those associated with centrosomal function may result in greater genome instability, thus driving the evolution of aggressively growing and high-grade cancer cells. The data thus verified the association of several known genes with breast tumorigenesis and uncovered additional novel associations, which together may underlie the molecular basis of current tumor grading systems in breast cancer.

The question of whether unique gene expression changes are associated with stage progression, specifically, the transition from noninvasive (DCIS) to invasive (IDC) growth, is also addressed by the present invention. The inventors have noticed that these two pathological stages are highly similar to each other with no striking differences at the level of gene expression (FIGS. 2-3). To increase our sensitivity in detecting differential gene expression between DCIS and IDC, each IDC sample was compared directly to its corresponding patient-matched DCIS sample where available. 1,688 genes showing at least a 2-fold difference between IDC and DCIS in at least 3 different sample pairs were selected and subjected to unsupervised two-dimensional hierarchical clustering. One prominent cluster of genes demonstrated elevated expression in LDC as compared with DCIS, predominately amongst the grade III IDC samples (FIG. 4). These genes, along with their I.M.A.G.E. Consortium CloneID number, along with their chromosomal location and descriptive identifiers (if known) are listed in Table 10.

TABLE 10 IMAGE Chromosome Clone ID Location Description 795498 15q26.1 HS1-2 | putative transmembrane protein 431505 15q26.1 HS1-2 | putative transmembrane protein 741139 20q13.1 EYA2 | eyes absent (Drosophila) homolog 2 1534592 2p12 C2orf6 | chromosome 2 open reading frame 6 290422 9q13-q21 ZNF216 | zinc finger protein 216 1609836 1q31 GLUL | glutamate-ammonia ligase (glutamine synthase) 505575 2q35 FLJ10116 | hypothetical protein FLJ10116 141852 11q13.5-q14.1 P2RY2 | purinergic receptor P2Y, G-protein coupled, 2 121251 12q13.1 MGC5576 | hypothetical protein MGC5576 610326-10 12q12-12q14.3 K-ALPHA-1 | tubulin, alpha, ubiquitous 725454 9q22 CKS2 | CDC28 protein kinase 2 756502 7p22 NUDT1 | nudix (nucleoside diphosphate linked moiety X)-type motif 1 504308 10cen-q26.11 FLJ10540 | hypothetical protein FLJ10540 2062329 6q13-q21 TTK | TTK protein kinase 564981 18 Homo sapiens, Similar to RIKEN cDNA 2810433K01 gene, clone MGC: 10200 IMAGE: 3909951, mRNA, complete cds 951080 8q24.3 RECQL4 | RecQ protein-like 4 280375 8p22 PRO2000 | PRO2000 protein 530219 8 Homo sapiens cDNA FLJ32554 fis, clone SPLEN1000106 594438 1q12-1q21.2 DJ328E19.C1.1 | hypothetical protein 470232 7 ESTs, Weakly similar to I37356 epithelial microtubule-associated protein, 115K [H. sapiens] 291057 1p32 CDKN2C | cyclin-dependent kinase inhibitor 2C (p18, inhibits CDK4) 1476053 15q15.1 RAD51 | RAD51 (S. cerevisiae) homolog (E coli RecA homolog) 121436 2q11.2 MGC4677 | hypothetical protein MGC4677 700792 14q22 CDKN3 | cyclin-dependent kinase inhibitor 3 (CDK2-associated dual specificity phosphatase) 308633 10q23-q24 HELLS | helicase, lymphoid-specific 809588 8q12.1 GGH | gamma-glutamyl hydrolase (conjugase, folylpolygammaglutamyl hydrolase) 1455394 7p15.2 HCS | cytochrome c 796694 17q25 BIRC5 | baculoviral IAP repeat-containing 5 (survivin) 2018131 12p13.2-p13.1 RACGAP1 | Rac GTPase activating protein 1 1587847 2q21 MCM6 | minichromosome maintenance deficient (mis5, S. pombe) 6 743810 12p13 MGC2577 | hypothetical protein MGC2577 744047 16p12.3 PLK | polo (Drosophila)-like kinase 705064 4p16.3 TACC3 | transforming, acidic coiled-coil containing protein 3 1518591 810899 ESTs 2018976 5q35.1 PTTG1 | pituitary tumor-transforming 1 2017415 2p24-p21 CENPA | centromere protein A (17 kD) 815501 19p13.3 MGC2721 | hypothetical protein MGC2721 624627 2p25-p24 RRM2 | ribonucleotide reductase M2 polypeptide 1422338 2p25-p24 RRM2 | ribonucleotide reductase M2 polypeptide 610326-8 12q12-12q14.3 K-ALPHA-1 | tubulin, alpha, ubiquitous 79761 12q22 TMPO | thymopoietin 610326-2 12q12-12q14.3 K-ALPHA-1 | tubulin, alpha, ubiquitous 610326-4 12q12-12q14.3 K-ALPHA-1 | tubulin, alpha, ubiquitous 610326-3 12q12-12q14.3 K-ALPHA-1 | tubulin, alpha, ubiquitous 1476065 1p36.1-p35 STMN1 | stathmin 1/oncoprotein 18 293785 11 ESTs, Weakly similar to A46010 X-linked retinopathy protein [H. sapiens] 47781 17 TEM7 | tumor endothelial marker 7 precursor 415102 5q31 CDC25C | cell division cycle 25C 869375 15q26.1 IDH2 | isocitrate dehydrogenase 2 (NADP+), mitochondrial 951241 15q13.3 ANKT | nucleolar protein ANKT 814270 4q27 PMSCL1 | polymyositis/scleroderma autoantigen 1 (75 kD) 785368 8p21-p12 TOPK | PDZ-binding kinase; T-cell originated protein kinase 66406 2 ESTs, Highly similar to T47163 hypothetical protein DKFZp762E1312.1 [H. sapiens] 292936 1p34.3 FLJ10468 | hypothetical protein FLJ10468 1517595 9p11.2 KIAA0175 | likely ortholog of maternal embryonic leucine zipper kinase 128711 7p15-p14 ANLN | anillin (Drosophila Scraps homolog), actin binding protein 200402 20q11.22-q12 DJ616B8.3 | hypothetical protein dJ616B8.3 825470 17q21-q22 TOP2A | topoisomerase (DNA) II alpha (170 kD) 769890 14q13.1 NP | nucleoside phosphorylase 796469 1q32.1 HSPC150 | HSPC150 protein similar to ubiquitin-conjugating enzyme 531319 17p13.1 STK12 | serine/threonine kinase 12 1416055 8 KIAA0165 | extra spindle poles, S. cerevisiae, homolog of 769921 20q13.12 UBE2C | ubiquitin-conjugating enzyme E2C 770992 839682 12q22 UBE2N | ubiquitin-conjugating enzyme E2N (homologous to yeast UBC13) 840364 20cen-q13.1 AHCY | S-adenosylhomocysteine hydrolase 276915 20q11.2 DNMT3B | DNA (cytosine-5-)-methyltransferase 3 beta

Interestingly, many of the genes in this duster have been identified already within the grade III signature cluster (FIG. 3). These include genes involved in the cell cycle (e.g., MCM6, TOP2A, CKS2, CDC25C), centrosomal function (TACC3, CENPA), and DNA repair (RAD51, RRM2). Thus, a subset of genes that are expressed at high levels in grade III DCIS are further elevated in IDC, suggesting an intriguing link between the two lines of cancer progression, i.e., tumor grade and invasion. Indeed, and without being bound by theory, RRM2, the M2 subunit of ribonucleotide reductase (RR), which catalyzes a rate-limiting step in DNA synthesis and repair, may play a dual role in both proliferative growth and invasion; overexpression of RRM2 in human cancer cells enhances their invasive potential (Zhou, B. S. et al. (1998e)), whereas its decreased expression inhibits cancer cell proliferation (Chen, S. et al., (2000)). In addition, centrosome amplification (e.g., induced by overexpression of STK15, Zhou et al. 1998b) may result in both high tumor grade and increased invasion potential due to altered cytoskeletal architecture (Lingle, W. L. et al.). However, these genes are not associated with the transition of grade I DCIS to grade I IDC, suggesting that the latter may employ a different mechanism(s) to gain invasion potential.

Without being bound by theory, and offered for the purposes of improving the understanding of the present invention and its possible applications, the above LCM-derived gene expression profiles of the various phenotypic stages of breast cancer are consistent with a modified model of breast cancer progression (FIG. 5). In this model, breast cancer develops along two dimensions, one of which consists of stage transitions from normal to ADH to DCIS to IDC and another consists of tumor grade progression from grade I to II to III. This model is supported by existing histopathological and clinical data (see Dupont, W. D. et al.; Marshall, L. M. et al.; Betsill, W. L. et al.; and Page, D. L. et al. (1982)) and the following lines of evidence presented above. First, extensive changes in gene expression occur in ADH and persist in DCIS/IDC, suggesting a molecular linkage between ADH and DCIS/IDC. Second, the identified 200 genes whose expression levels quantitatively correlate with tumor grade progression in both DCIS and IDC indicate a transcriptional continuum from low to high-grade tumors. Finally, grade III DCIS and DC differ quantitatively in the expression of the same genes associated with tumor grade progression. It is thus proposed that the various subtypes (e.g., ER+ and ER− subtypes) of breast cancer represent snapshots of this two-dimensional progression scheme; for example (and without limiting the invention), during the progression from grade I through grade III, ER-positive lesions evolve into ER-negative ones. The present invention thus provides the identity, and thus sequences, of various genes associated with the initiation and progression of breast cancer, and so provides for novel diagnostic, preventative and therapeutic strategies for women with breast cancer. This includes the ability to utilize the grade of DCIS/IDC breast cancer, irrespective of which stage of breast cancer is actually present, as a criterion for decisions concerning breast cancer diagnosis and treatment.

The following Table 11 summarizes the contents of Tables 2-10

TABLE 11 Table Description 2 Genes with elevated expression in ADH and persisting through DCIS and IDC cells compared to normal cells 3 Genes with highest expression in grade III DCIS or IDC cells 4 Genes with decreased expression in ADH, DCIS and IDC cells compared to normal cells 5 Genes correlated with grade I and III samples and decreased expression in all samples 6 Genes with increased expression in grade III (DCIS and/or IDC) samples 7 Genes with increased expression in grade I (DCIS and/or IDC) samples 8 250 genes with increased expression in grade I (DCIS and/or IDC) samples 9 250 genes with increased expression in grade III (DCIS and/or IDC) samples 10 Genes with quantitative differences in expression between DCIS and IDC samples

Having now generally described the invention, the same will be more readily understood through reference to the following examples which are provided by way of illustration, and are not intended to be limiting of the present invention, unless specified.

EXAMPLES Example I Materials and Methods

Clinical specimen collection and clinicopathological parameters. All breast specimens were obtained from the Massachusetts General Hospital between 1998 and 2001. Thirty-six breast cancer patients were selected, 31 of which were diagnosed with two or more pathological stages of breast cancer progression, and 5 of which were diagnosed with pre-invasive disease only. Three healthy women who underwent elective mammoplasty reduction were selected as disease-free normal controls. Tissue specimens that demonstrated one or more pathological lesions (ADH, DCIS and IDC) were selected for the study. Cases of ADH were selected as proliferative epithelial lesions that possessed some, but not all, of the features of carcinoma in situ (Page, D. L, et al. (1992)) and most closely resemble those lesions described as CAPSS (Oyama, T. et al, and Fraser, J. L. et al.). DCIS and IDC were classified (histological grade) according to the European classification (Holland, R. et al.) and by the. Nottingham combined histological grade (Elston, C. W. et al.), respectively. ER and PR expression were determined by immunohistochemical staining (negative when none of the tumor cell nuclei showed staining), and Her-2 expression determined by immunohistochemistry or FISH. This study was approved the Massachusetts General Hospital human research committee in accordance with NIH human research study guidelines.

LCM and RNA isolation and amplification. Each component (Normal, ADH, DCIS or IDC) was laser capture microdissected in triplicate (from consecutive tissue sections) as described (Sgroi et al.) using a PixCell II LCM system (Arcturus Engineering Inc., Mountain View, Calif.). Total RNA was extracted from the captured cells using the Picopure™ RNA Isolation Kit (Arcturus). T7-based RNA amplification was carried out using the RiboAmp™ kit (Arcturus). Briefly, the RNA from each sample was primed with an oligo-dT primer containing a T7 promoter sequence, reverse transcribed and then converted to double stranded cDNA. The cDNA templates were then used in an in vitro transcription reaction using T7 RNA polymerase to generate amplified RNA (aRNA). To obtain enough aRNA for a microarray experiment, a second round of RNA amplification was performed on all samples. To serve as reference in microarray hybridizations, a human universal reference RNA from Stratagene (La Jolla, Calif.) was amplified identically.

Fabrication of microarrays. Sequence-verified human cDNA clones were obtained from Research Genetics (Huntsville, Ala.). cDNA clones (from the I.M.A.G.E. Consortium via Research Genetics) inserts were amplified by PCR, gel-purified, and spotted onto a 1×3-inch SuperAmine™ (TeleChem International, Sunnyvale, Calif.) glass microscope slide using an OmniGrid™ robotic arrayer (GeneMachines, San Carlos, Calif.). As used herein, the I.M.A.G.E. Consortium CloneID, or the IMAGE CloneID, lists the identifiers of the cDNA clones on the microarrays according to the I.M.A.G.E. Consortium and Research Genetics (www.resgen.com/). This provides a unique single identifier for each clone. Descriptive names of clones (or genes) use the UniGene symbols and titles (www.ncbi.nlm.nih.gov/UniGene/).

Probe labeling and hybridization. cDNA was transcribed from aRNA in the presence of 5-(3-aminoallyl)-2′-deoxyuridine 5′-triphosphate (aminoallyl dUTP) using Stratagene's FairPlay Kit™ (La Jolla, Calif.). Cy3 or Cy5 mono-reactive dye (Amersham, Piscataway, N.J.) was conjugated onto purified cDNA and the residual dye was removed using QiaQuick PCR Purification columns (Qiagen, Valencia, Calif.). Each Cy5-labeled cDNA was hybridized together with the Cy3-labeled reference probe to a microarray in 40 μL hybridization solution (5×SSC, 0.1 μg/μL COT I, 0.2% SDS, 50% formamide) at a concentration of 25 ng/μL per channel for 17 hrs at 42° C. in >60% relative humidity.

Washing, scanning and image analysis. After hybridization, slides were washed as follows: 1×SSC, 0.2% SDS at 42° for 5 min (two times), 1×SSC, 0.2% SDS at 55° C. for 5 min, 0.1×SSC, 0.2% SDS at 55° C. for 5 min and 0.1×SSC at RT for 2 min. Washed slides were scanned using ScanArray 5000 (PerkinElmer, Billerica, Mass.), and Cy5/Cy3-signals were quantitated using ImaGene 4.2 (BioDiscovery, Los Angeles, Calif.).

Data processing. Fluorescent intensities of Cy5 and Cy3 channels on each slide were subjected to spot filtering and normalization. Spots flagged by ImaGene were excluded from further analysis. Normalization was performed using a robust nonlinear local regression method (Yang, Y. H. et al.). The normalized ratios of Cy5/Cy3 were used to represent the relative gene expression levels in the experimental samples. Measurements from replicate samples were averaged after normalization.

Cluster and discriminant analysis. Hierarchical cluster analysis was performed in GeneMaths (v1.5, Applied-Maths, Austin, Tex.) using the cosine correlation coefficient as a measure of similarity between two genes or samples and complete linkage. Linear discriminant analysis with variance was performed within GeneMaths.

Example II Genes Showing Significant Differences in the Pair-wise Comparisons of Normal vs. ADH, Normal vs. DCIS and Normal vs. IDC by Linear Discriminant Analysis

2-3 independent LCM captures were made from the same breast biopsy for each disease state (normal, ADH, DOS or IDC), and RNA from each capture was amplified, labeled, and hybridized to 2 identical 12,000-element microarrays, resulting in from 4 to 6 data points per gene per disease state. The replicate data points were averaged to represent the expression level of each gene at each cellular state, which was further transformed as data points which are the log 2 value of the ratio of data from patient matched disease/normal samples or the log 2 value of the ratio of data from patient matched IDC/DCIS samples.

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All references cited herein, including patents, patent applications, and publications, are hereby incorporated by reference in their entireties, whether previously specifically incorporated or not.

Having now Wily described this invention, it will be appreciated by those skilled in the art that the same can be performed within a wide range of equivalent parameters, concentrations, and conditions without departing from the spirit and scope of the invention and without undue experimentation.

While this invention has been described in connection with specific embodiments thereof, it will be understood that it is capable of further modifications. This application is intended to cover any variations, uses, or adaptations of the invention following, in general, the principles of the invention and including such departures from the present disclosure as come within known or customary practice within the art to which the invention pertains and as may be applied to the essential features hereinbefore set forth. 

The invention claimed is:
 1. A method of treating breast cancer in a human subject, said method comprising assaying a sample from the human subject for gene expression levels of CENPA (centromere protein A (17 kD), chromosomal location 2p24-p21), RACGAP1 (Rac GTPase activating protein 1, chromosomal location 12p13.2-p13.1), RRM2 (ribonucleotide reductase M2 polypeptide, chromosomal location 2p25-p24), and NEK2 (NIMA (never in mitosis gene a)-related kinase, chromosomal location 1q32.2-q41); determining a measure of similarity between the gene expression levels of the human subject and reference gene expression levels for a reference population of cancer subjects; and either (a) treating the human subject with an antitumor agent, chemotherapy, or surgical removal of cancer tissue if the measure of similarity is above a threshold; or (b) conducting a cytological examination of cells from the human subject if the measure of similarity is above the threshold.
 2. The method of claim 1 wherein said assaying comprises amplifying RNA from said sample.
 3. The method of claim 2 wherein amplifying said RNA comprises quantitative PCR amplification.
 4. The method of claim 2 wherein amplifying said RNA comprises reverse transcription PCR (RT-PCR).
 5. The method of claim 1 wherein said assaying comprises determining gene expression levels by array hybridization.
 6. The method of claim 1 wherein said sample is a ductal lavage, needle biopsy, surgical biopsy, or fine needle aspirate sample.
 7. The method of claim 1, wherein said sample is microdissected to isolate one or more cells suspected of being breast cancer cells and said assaying is of RNA in said isolated cells.
 8. A method of treating breast cancer in a human subject, said method comprising assaying a sample from the human subject for gene expression levels of CENPA (centromere protein A (17 kD), chromosomal location 2p24-p21), RACGAP1 (Rac GTPase activating protein 1, chromosomal location 12p13.2-p13.1), RRM2 (ribonucleotide reductase M2 polypeptide, chromosomal location 2p25-p24), and NEK2 (NIMA (never in mitosis gene a)-related kinase, chromosomal location 1q32.2-q41); comparing the gene expression levels of the human subject to corresponding reference gene expression levels for a reference population of cancer subjects; and either (a) treating the human subject with chemotherapy if the gene expression levels of the human subject are higher than the corresponding reference gene expression levels, (b) conducting a cytological examination of cells from the human subject if the gene expression levels of the human subject are higher than the corresponding reference gene expression levels, or (c) administering a breast cancer treatment other than chemotherapy if the gene expression levels of the human subject are lower than the corresponding reference gene expression levels.
 9. The method of claim 8 wherein said assaying comprises amplifying RNA from said sample.
 10. The method of claim 9 wherein amplifying said RNA comprises quantitative PCR amplification.
 11. The method of claim 9 wherein amplifying said RNA comprises reverse transcription PCR (RT-PCR).
 12. The method of claim 8 wherein said assaying comprises determining gene expression levels by array hybridization.
 13. The method of claim 8 wherein said sample is a ductal lavage, needle biopsy, surgical biopsy, or fine needle aspirate sample.
 14. The method of claim 8 wherein said sample is microdissected to isolate one or more cells suspected of being breast cancer cells and said assaying is of RNA in said isolated cells.
 15. The method of claim 1, wherein the human subject is treated with chemotherapy if the measure of similarity is above the threshold.
 16. The method of claim 8, wherein the human subject is treated with chemotherapy if the gene expression levels of the human subject are higher than the corresponding reference gene expression levels. 